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胰高血糖素样肽I通过增强细胞内钙动员增加胰岛素分泌β TC3细胞中的细胞质钙。

Glucagon-like peptide I increases cytoplasmic calcium in insulin-secreting beta TC3-cells by enhancement of intracellular calcium mobilization.

作者信息

Gromada J, Dissing S, Bokvist K, Renström E, Frøkjaer-Jensen J, Wulff B S, Rorsman P

机构信息

Department of Medical Physiology, Panum Institute, University of Copenhagen, Denmark.

出版信息

Diabetes. 1995 Jul;44(7):767-74. doi: 10.2337/diab.44.7.767.

DOI:10.2337/diab.44.7.767
PMID:7789644
Abstract

In the insulin-secreting beta-cell line beta TC3, stimulation with 11.2 mmol/l glucose caused a rise in the intracellular free Ca2+ concentration ([Ca2+]i) in only 18% of the tested cells. The number of glucose-responsive cells increased after pretreatment of the cells with glucagon-like peptide I (GLP-I)(7-36)amide and at 10(-11) mol/l; 84% of the cells responded to glucose with a rise in [Ca2+]i. GLP-I(7-36)amide induces a rapid increase in [Ca2+]i only in cells exposed to elevated glucose concentrations (> or = 5.6 mmol/l). The action of GLP-I(7-36)amide and forskolin involved a 10-fold increase in cytoplasmic cAMP concentration and was mediated by activation of protein kinase A. It was not associated with an effect on the membrane potential but required some (small) initial entry of Ca2+ through voltage-dependent L-type Ca2+ channels, which then produced a further increase in [Ca2+]i by mobilization from intracellular stores. The latter effect reflected Ca(2+)-induced Ca2+ release and was blocked by ryanodine. Similar increases in [Ca2+]i were also observed in voltage-clamped cells, although there was neither activation of a background (Ca(2+)-permeable) inward current nor enhancement of the voltage-dependent L-type Ca2+ current. These observations are consistent with GLP-I(7-36) amide inducing glucose sensitivity by promoting mobilization of Ca2+ from intracellular stores. We propose that this novel action of GLP-I(7-36)amide represents an important factor contributing to its insulinotropic action.

摘要

在分泌胰岛素的β细胞系βTC3中,用11.2 mmol/l葡萄糖刺激时,仅18%的受试细胞细胞内游离Ca2+浓度([Ca2+]i)升高。用胰高血糖素样肽I(GLP-I)(7-36)酰胺预处理细胞后,葡萄糖反应性细胞数量增加,在10(-11) mol/l时,84%的细胞对葡萄糖反应时[Ca2+]i升高。GLP-I(7-36)酰胺仅在暴露于高葡萄糖浓度(≥5.6 mmol/l)的细胞中诱导[Ca2+]i快速增加。GLP-I(7-36)酰胺和福司可林的作用涉及细胞质cAMP浓度增加10倍,由蛋白激酶A激活介导。它与对膜电位的影响无关,但需要一些(少量)Ca2+通过电压依赖性L型Ca2+通道的初始内流,然后通过从细胞内储存库中动员进一步增加[Ca2+]i。后一种效应反映了Ca(2+)诱导的Ca2+释放,并被ryanodine阻断。在电压钳制的细胞中也观察到了类似的[Ca2+]i增加,尽管既没有背景(Ca(2+)可渗透)内向电流的激活,也没有电压依赖性L型Ca2+电流的增强。这些观察结果与GLP-I(7-36)酰胺通过促进细胞内储存库中Ca2+的动员诱导葡萄糖敏感性一致。我们提出,GLP-I(7-36)酰胺的这种新作用代表了其促胰岛素作用的一个重要因素。

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