Maechler P, Kennedy E D, Sebö E, Valeva A, Pozzan T, Wollheim C B
Division of Clinical Biochemistry and Experimental Diabetology, Department of Internal Medicine, University Medical Center, CH-1211 Geneva 4, Switzerland.
J Biol Chem. 1999 Apr 30;274(18):12583-92. doi: 10.1074/jbc.274.18.12583.
The precise regulation of the Ca2+ concentration in the endoplasmic reticulum ([Ca2+]er) is important for protein processing and signal transduction. In the pancreatic beta-cell, dysregulation of [Ca2+]er may cause impaired insulin secretion. The Ca2+-sensitive photoprotein aequorin mutated to lower its Ca2+ affinity was stably expressed in the endoplasmic reticulum (ER) of rat insulinoma INS-1 cells. The steady state [Ca2+]er was 267 +/- 9 microM. Both the Ca2+-ATPase inhibitor cyclopiazonic acid and 4-chloro-m-cresol, an activator of ryanodine receptors, caused an almost complete emptying of ER Ca2+. The inositol 1,4,5-trisphosphate generating agonists, carbachol, and ATP, reduced [Ca2+]er by 20-25%. Insulin secretagogues that raise cytosolic [Ca2+] by membrane depolarization increased [Ca2+]er in the potency order K+ >> glucose > leucine, paralleling their actions in the cytosolic compartment. Glucose, which augmented [Ca2+]er by about 25%, potentiated the Ca2+-mobilizing effect of carbachol, explaining the corresponding observation in cytosolic [Ca2+]. The filling of ER Ca2+ by glucose is not directly mediated by ATP production as shown by the continuous monitoring of cytosolic ATP in luciferase expressing cells. Both glucose and K+ increase [Ca2+]er, but only the former generated whereas the latter consumed ATP. Nonetheless, drastic lowering of cellular ATP with a mitochondrial uncoupler resulted in a marked decrease in [Ca2+]er, emphasizing the requirement for mitochondrially derived ATP above a critical threshold concentration. Using alpha-toxin permeabilized cells in the presence of ATP, glucose 6-phosphate did not change [Ca2+]er, invalidating the hypothesis that glucose acts through this metabolite. Therefore, insulin secretagogues that primarily stimulate Ca2+ influx, elevate [Ca2+]er to ensure beta-cell homeostasis.
内质网中钙离子浓度([Ca2+]er)的精确调节对于蛋白质加工和信号转导至关重要。在胰腺β细胞中,[Ca2+]er失调可能导致胰岛素分泌受损。将对Ca2+亲和力降低的Ca2+敏感光蛋白水母发光蛋白稳定表达于大鼠胰岛素瘤INS-1细胞的内质网(ER)中。稳态[Ca2+]er为267±9微摩尔。Ca2+-ATP酶抑制剂环匹阿尼酸和ryanodine受体激活剂4-氯间甲酚均可导致内质网Ca2+几乎完全排空。生成肌醇1,4,5-三磷酸的激动剂、卡巴胆碱和ATP可使[Ca2+]er降低20%-25%。通过膜去极化提高胞质[Ca2+]的胰岛素促分泌剂按K+>>葡萄糖>亮氨酸的效力顺序增加[Ca2+]er,这与它们在胞质区室中的作用平行。使[Ca2+]er增加约25%的葡萄糖增强了卡巴胆碱的Ca2+动员作用,这解释了在胞质[Ca2+]中的相应观察结果。如在表达荧光素酶的细胞中对胞质ATP的连续监测所示,葡萄糖对内质网Ca2+的填充并非直接由ATP生成介导。葡萄糖和K+均可增加[Ca2+]er,但只有前者生成而后者消耗ATP。尽管如此,用线粒体解偶联剂大幅降低细胞ATP会导致[Ca2+]er显著降低,强调了高于临界阈值浓度的线粒体衍生ATP的需求。在有ATP存在的情况下使用α-毒素通透细胞,6-磷酸葡萄糖不会改变[Ca2+]er,这使葡萄糖通过这种代谢物起作用的假设不成立。因此,主要刺激Ca2+内流的胰岛素促分泌剂会升高[Ca2+]er以确保β细胞内环境稳定。
