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葡萄糖刺激胰腺β细胞系可诱导强啡肽的表达与分泌。

Glucose stimulation of pancreatic beta-cell lines induces expression and secretion of dynorphin.

作者信息

Josefsen K, Buschard K, Sørensen L R, Wøllike M, Ekman R, Birkenbach M

机构信息

Bartholin Instituttet, Kommunehospitalet, Copenhagen K, Denmark.

出版信息

Endocrinology. 1998 Oct;139(10):4329-36. doi: 10.1210/endo.139.10.6233.

Abstract

To investigate adaptive responses of pancreatic beta-cells to hyperglycemia, genes induced by glucose stimulation were identified by subtraction cloning. Among 53 clones representing differentially expressed genes, 20 encoded the endogenous opioid precursor, prodynorphin. The amino acid sequence of murine prodynorphin is identical to the rat protein in sequences comprising the opioid peptides and 86% identical in the remainder of the molecule. Stimulation of MIN6 cells increased prodynorphin RNA levels to more than 20-fold in proportion to physiological glucose concentrations. Similar induction levels were observed in murine betaTC3 and rat Rinm5F beta-cell lines. Prodynorphin RNA expression increased within 1 h of glucose stimulation, achieved maximal levels by 4 h, and remained elevated for at least 24 h. By using RIA, MIN6 cells were shown to contain and secrete increased amounts of dynorphin-A following glucose stimulation. Treatment of MIN6 cells with KCl, forskolin, or isobutyl-methyl-xanthine strongly induced prodynorphin RNA expression, suggesting that induction may be related to secretion-coupled signaling pathways. The induction of prodynorphin in several beta-cell lines is consistent with previous demonstrations of beta-cell synthesis of other endogenous opioids, including beta-endorphin, and suggests that opioids may have a potentially significant role in regulating beta-cell secretion.

摘要

为研究胰腺β细胞对高血糖的适应性反应,通过消减克隆鉴定了葡萄糖刺激诱导的基因。在代表差异表达基因的53个克隆中,20个编码内源性阿片肽前体强啡肽原。小鼠强啡肽原的氨基酸序列在包含阿片肽的序列中与大鼠蛋白相同,在分子其余部分有86%的同源性。刺激MIN6细胞可使强啡肽原RNA水平随着生理葡萄糖浓度的升高而增加至20倍以上。在小鼠βTC3和大鼠Rinm5Fβ细胞系中也观察到类似的诱导水平。葡萄糖刺激1小时内强啡肽原RNA表达增加,4小时达到最高水平,并至少持续升高24小时。通过放射免疫分析显示,葡萄糖刺激后MIN6细胞中强啡肽A的含量和分泌量增加。用氯化钾、福斯可林或异丁基甲基黄嘌呤处理MIN6细胞可强烈诱导强啡肽原RNA表达,提示这种诱导可能与分泌偶联信号通路有关。几种β细胞系中强啡肽原的诱导与先前β细胞合成其他内源性阿片肽(包括β-内啡肽)的研究结果一致,表明阿片肽可能在调节β细胞分泌中具有潜在的重要作用。

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