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定量NAD(P)H/黄素蛋白自发荧光成像揭示胰岛丙酮酸反应的代谢机制。

Quantitative NAD(P)H/flavoprotein autofluorescence imaging reveals metabolic mechanisms of pancreatic islet pyruvate response.

作者信息

Rocheleau Jonathan V, Head W Steven, Piston David W

机构信息

Molecular Physiology and Biophysics, Vanderbilt University, Nashville, Tennessee 37232, USA

出版信息

J Biol Chem. 2004 Jul 23;279(30):31780-7. doi: 10.1074/jbc.M314005200. Epub 2004 May 17.


DOI:10.1074/jbc.M314005200
PMID:15148320
Abstract

Glucose-stimulated insulin secretion is a multistep process dependent on beta-cell metabolic flux. Our previous studies on intact pancreatic islets used two-photon NAD(P)H imaging as a quantitative measure of the combined redox signal from NADH and NADPH (referred to as NAD(P)H). These studies showed that pyruvate, a non-secretagogue, enters beta-cells and causes a transient rise in NAD(P)H. To further characterize the metabolic fate of pyruvate, we have now developed one-photon flavoprotein microscopy as a simultaneous assay of lipoamide dehydrogenase (LipDH) autofluorescence. This flavoprotein is in direct equilibrium with mitochondrial NADH. Hence, a comparison of LipDH and NAD(P)H autofluorescence provides a method to distinguish the production of NADH, NADPH, or both. Using this method, the glucose dose response is consistent with an increase in both NADH and NADPH. In contrast, the transient rise in NAD(P)H observed with pyruvate stimulation is not accompanied by a significant change in LipDH, which indicates that pyruvate raises cellular NADPH without raising NADH. In comparison, methyl pyruvate stimulated a robust NADH and NADPH response. These data provide new evidence that exogenous pyruvate does not induce a significant rise in mitochondrial NADH. This inability likely results in its failure to produce the ATP necessary for stimulated secretion of insulin. Overall, these data are consistent with either a restricted pyruvate dehydrogenase-dependent metabolism or a buffering of the NADH response by other metabolic mechanisms.

摘要

葡萄糖刺激的胰岛素分泌是一个依赖于β细胞代谢通量的多步骤过程。我们之前对完整胰岛的研究使用双光子NAD(P)H成像作为来自NADH和NADPH(称为NAD(P)H)的组合氧化还原信号的定量测量。这些研究表明,丙酮酸,一种非促分泌剂,进入β细胞并导致NAD(P)H短暂升高。为了进一步表征丙酮酸的代谢命运,我们现在开发了单光子黄素蛋白显微镜作为硫辛酰胺脱氢酶(LipDH)自发荧光的同步测定方法。这种黄素蛋白与线粒体NADH直接处于平衡状态。因此,比较LipDH和NAD(P)H自发荧光提供了一种区分NADH、NADPH或两者产生的方法。使用这种方法,葡萄糖剂量反应与NADH和NADPH的增加一致。相比之下,丙酮酸刺激观察到的NAD(P)H短暂升高并未伴随着LipDH的显著变化,这表明丙酮酸升高细胞NADPH而不升高NADH。相比之下,丙酮酸甲酯刺激了强烈的NADH和NADPH反应。这些数据提供了新的证据,即外源性丙酮酸不会诱导线粒体NADH的显著升高。这种无能可能导致其无法产生刺激胰岛素分泌所需的ATP。总体而言,这些数据与丙酮酸脱氢酶依赖性代谢受限或其他代谢机制对NADH反应的缓冲作用一致。

相似文献

[1]
Quantitative NAD(P)H/flavoprotein autofluorescence imaging reveals metabolic mechanisms of pancreatic islet pyruvate response.

J Biol Chem. 2004-7-23

[2]
Pancreatic islet beta-cells transiently metabolize pyruvate.

J Biol Chem. 2002-8-23

[3]
Quantitative imaging of electron transfer flavoprotein autofluorescence reveals the dynamics of lipid partitioning in living pancreatic islets.

Integr Biol (Camb). 2012-6-25

[4]
Ca2+ controls slow NAD(P)H oscillations in glucose-stimulated mouse pancreatic islets.

J Physiol. 2006-4-15

[5]
Cytosolic ratios of free [NADPH]/[NADP+] and [NADH]/[NAD+] in mouse pancreatic islets, and nutrient-induced insulin secretion.

Biochem J. 1987-1-1

[6]
Feasibility of a mitochondrial pyruvate malate shuttle in pancreatic islets. Further implication of cytosolic NADPH in insulin secretion.

J Biol Chem. 1995-8-25

[7]
Methyl pyruvate stimulates pancreatic beta-cells by a direct effect on KATP channels, and not as a mitochondrial substrate.

Biochem J. 2002-12-15

[8]
Acute metabolic amplification of insulin secretion in mouse islets is mediated by mitochondrial export of metabolites, but not by mitochondrial energy generation.

Metabolism. 2013-6-18

[9]
Role of NADH shuttle system in glucose-induced activation of mitochondrial metabolism and insulin secretion.

Science. 1999-2-12

[10]
Effect of Methylene Blue on pyridine nucleotides and insulin secretion of rat pancreatic islets.

Diabetologia. 1979-7

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[3]
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[10]
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