Urzì Christian, Meyer Christoph, Mathis Déborah, Vermathen Peter, Nuoffer Jean-Marc
Magnetic Resonance Methodology, Institute of Diagnostic and Interventional Neuroradiology, University of Bern, Bern, Switzerland.
University Institute of Clinical Chemistry, Inselspital, Bern University Hospital, Bern, Switzerland.
J Inherit Metab Dis. 2025 Jan;48(1):e12794. doi: 10.1002/jimd.12794. Epub 2024 Sep 4.
Metabolomic discrimination of different mitochondrial defects is challenging. We describe an NMR-based bioreactor allowing real-time intra- and extracellular metabolic investigation of perfused fibroblasts.
The objective of this study is (I) determining whether metabolic investigations of perfused fibroblasts overall and separated for intra- and extracellular contributions by real-time NMR allows for discrimination of different representative mitochondrial defects in a feasibility study and (II) gaining insight into physiological consequences of mitochondrial dysfunction in basal condition and during glycolysis inhibition.
Overall, intra- and extracellular metabolomes of malate dehydrogenase 2 (MDH2), pyruvate dehydrogenase (PDH), complex I (CI) deficient fibroblasts, and control fibroblasts were investigated under standard culture conditions and under glycolysis inhibition. In addition to "overall" metabolite quantification, intra- and extracellular metabolic contributions were separated based on diffusion rate differences.
Overall metabolites: Chemometric analysis of the entire metabolome revealed good separation between control, PDH and MDH2, while CI was less well separated. However, mixed intra- and extracellular changes complicated interpretation of the cellular metabolism. Intra- and extracellular metabolites: Compartment specific chemometrics revealed possibly augmenting metabolomic separation between control and deficient cell lines under basal and inhibition condition. All mitochondrial defects exhibited upregulation of glycolytic metabolism compared to controls. Inhibition of glycolysis resulted in perturbations of other metabolic pathways such as glutaminolysis, alanine, arginine, glutamate, and proline metabolism. MDH2 showed upregulation of alanine and glutamate metabolism, while the CI defect revealed lower intracellular arginine and downregulation of glutamate and arginine-dependent proline synthesis.
Discrimination of intra- and extracellular metabolic contributions helps understanding the underlying mechanisms of mitochondrial disorders, uncovers potential metabolic biomarkers, and unravels metabolic pathway-specific adaptations in response to metabolic perturbations.
对不同线粒体缺陷进行代谢组学区分具有挑战性。我们描述了一种基于核磁共振的生物反应器,可对灌注的成纤维细胞进行实时细胞内和细胞外代谢研究。
本研究的目的是:(I)在一项可行性研究中,确定通过实时核磁共振对灌注的成纤维细胞进行整体以及区分细胞内和细胞外贡献的代谢研究,是否能够区分不同的代表性线粒体缺陷;(II)深入了解基础状态下以及糖酵解抑制期间线粒体功能障碍的生理后果。
总体而言,在标准培养条件下以及糖酵解抑制条件下,研究了苹果酸脱氢酶2(MDH2)、丙酮酸脱氢酶(PDH)、复合体I(CI)缺陷的成纤维细胞以及对照成纤维细胞的细胞内和细胞外代谢组。除了“整体”代谢物定量外,还基于扩散速率差异分离了细胞内和细胞外的代谢贡献。
整体代谢物:对整个代谢组的化学计量学分析显示,对照组、PDH和MDH2之间有良好的区分,而CI的区分度较差。然而,细胞内和细胞外变化的混合使得对细胞代谢的解释变得复杂。细胞内和细胞外代谢物:特定区室的化学计量学显示,在基础和抑制条件下,对照组和缺陷细胞系之间的代谢组区分可能会增强。与对照组相比,所有线粒体缺陷均表现出糖酵解代谢上调。糖酵解抑制导致其他代谢途径受到干扰,如谷氨酰胺分解、丙氨酸、精氨酸、谷氨酸和脯氨酸代谢。MDH2表现出丙氨酸和谷氨酸代谢上调,而CI缺陷显示细胞内精氨酸含量较低,谷氨酸和精氨酸依赖性脯氨酸合成下调。
区分细胞内和细胞外代谢贡献有助于理解线粒体疾病的潜在机制,发现潜在的代谢生物标志物,并揭示代谢途径特异性对代谢干扰的适应性变化。
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