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使用新型荧光共振能量转移(FRET)生物传感器直接测量胰腺胰岛β细胞中丙酮酸激酶 M2 活性的振荡糖酵解。

Direct measurements of oscillatory glycolysis in pancreatic islet β-cells using novel fluorescence resonance energy transfer (FRET) biosensors for pyruvate kinase M2 activity.

机构信息

From the Department of Pharmacology and Brehm Center for Diabetes Research, University of Michigan Medical School, Ann Arbor, Michigan 48105.

出版信息

J Biol Chem. 2013 Nov 15;288(46):33312-22. doi: 10.1074/jbc.M113.508127. Epub 2013 Oct 7.

Abstract

Pulses of insulin released from pancreatic β-cells maintain blood glucose in a narrow range, although the source of these pulses is unclear. We and others have proposed that positive feedback mediated by the glycolytic enzyme phosphofructokinase-1 (PFK1) enables β-cells to generate metabolic oscillations via autocatalytic activation by its product fructose 1,6-bisphosphate (FBP). Although much indirect evidence has accumulated in favor of this hypothesis, a direct measurement of oscillating glycolytic intermediates has been lacking. To probe glycolysis directly, we engineered a family of inter- and intramolecular FRET biosensors based on the glycolytic enzyme pyruvate kinase M2 (PKAR; pyruvate kinase activity reporter), which multimerizes and is activated upon binding FBP. When introduced into Min6 β-cells, PKAR FRET efficiency increased rapidly in response to glucose. Importantly, however, metabolites entering downstream of PFK1 (glyceraldehyde, pyruvate, and ketoisocaproate) failed to activate PKAR, consistent with sensor activation by FBP; the dependence of PKAR on FBP was further confirmed using purified sensor in vitro. Using a novel imaging modality for monitoring mitochondrial flavin fluorescence in mouse islets, we show that slow oscillations in mitochondrial redox potential stimulated by 10 mm glucose are in phase with glycolytic efflux through PKM2, measured simultaneously from neighboring islet β-cells expressing PKAR. These results indicate that PKM2 activity in β-cells is oscillatory and are consistent with pulsatile PFK1 being the mediator of slow glycolytic oscillations.

摘要

尽管胰腺 β 细胞释放的胰岛素脉冲可以将血糖维持在狭窄范围内,但这些脉冲的来源尚不清楚。我们和其他人曾提出,糖酵解酶磷酸果糖激酶 1(PFK1)介导的正反馈使β细胞能够通过其产物果糖 1,6-二磷酸(FBP)的自动催化激活产生代谢振荡。尽管已经积累了大量支持这一假设的间接证据,但一直缺乏对振荡糖酵解中间产物的直接测量。为了直接探测糖酵解,我们设计了一系列基于糖酵解酶丙酮酸激酶 M2(PKAR;丙酮酸激酶活性报告物)的分子内和分子间的 FRET 生物传感器,该酶在结合 FBP 时多聚化并被激活。当将 PKAR FRET 效率引入 Min6 β 细胞时,其会快速响应葡萄糖而增加。然而,重要的是,进入 PFK1 下游的代谢物(甘油醛、丙酮酸和酮异己酸)未能激活 PKAR,这与 FBP 激活传感器一致;使用体外纯化的传感器进一步证实了 PKAR 对 FBP 的依赖性。使用一种新的成像方式来监测小鼠胰岛中线粒体黄素荧光的变化,我们发现,10mm 葡萄糖刺激的线粒体氧化还原电势的缓慢振荡与通过 PKM2 的糖酵解流出同步,同时从表达 PKAR 的相邻胰岛β细胞中测量。这些结果表明,β细胞中 PKM2 的活性是振荡的,并且与脉冲式 PFK1 作为缓慢糖酵解振荡的介导物一致。

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