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细胞氧化甲醛生成的甲酸盐可加速培养星形胶质细胞中的糖酵解通量。

Formate generated by cellular oxidation of formaldehyde accelerates the glycolytic flux in cultured astrocytes.

机构信息

Centre for Biomolecular Interactions Bremen, University of Bremen, Bremen, Germany.

出版信息

Glia. 2012 Apr;60(4):582-93. doi: 10.1002/glia.22292. Epub 2012 Jan 18.

DOI:10.1002/glia.22292
PMID:22258934
Abstract

Formaldehyde is a neurotoxic compound that can be endogenously generated in the brain. Because astrocytes play a key role in metabolism and detoxification processes in brain, we have investigated the capacity of these cells to metabolize formaldehyde using primary astrocyte-rich cultures as a model system. Application of formaldehyde to these cultures resulted in the appearance of formate in cells and in a time-, concentration- and temperature-dependent disappearance of formaldehyde from the medium that was accompanied by a matching extracellular accumulation of formate. This formaldehyde-oxidizing capacity of astrocyte cultures is likely to be catalyzed by alcohol dehydrogenase 3 and aldehyde dehydrogenase 2, because the cells of the cultures contain the mRNAs of these formaldehyde-oxidizing enzymes. In addition, exposure to formaldehyde increased both glucose consumption and lactate production by the cells. Both the strong increase in the cellular formate content and the increase in glycolytic flux were only observed after application of formaldehyde to the cells, but not after treatment with exogenous methanol or formate. The accelerated lactate production was not additive to that obtained for azide, a known inhibitor of complex IV of the respiratory chain, and persisted after removal of formaldehyde after a formaldehyde exposure for 1.5 h. These data demonstrate that cultured astrocytes efficiently oxidize formaldehyde to formate, which subsequently enhances glycolytic flux, most likely by inhibition of mitochondrial respiration.

摘要

甲醛是一种神经毒性化合物,可在大脑内内源性产生。由于星形胶质细胞在大脑的代谢和解毒过程中发挥关键作用,我们利用富含星形胶质细胞的原代培养物作为模型系统,研究了这些细胞代谢甲醛的能力。将甲醛应用于这些培养物中,导致细胞中出现甲酸盐,并且甲醛从培养基中以时间、浓度和温度依赖的方式消失,同时伴有甲酸盐的相应细胞外积累。星形胶质细胞培养物的这种甲醛氧化能力可能是由醇脱氢酶 3 和醛脱氢酶 2 催化的,因为培养物中的细胞含有这些甲醛氧化酶的 mRNA。此外,甲醛暴露增加了细胞的葡萄糖消耗和乳酸产生。只有在将甲醛应用于细胞后,才会观察到细胞中甲酸盐含量的强烈增加和糖酵解通量的增加,而在用外源性甲醇或甲酸盐处理后则不会观察到这种情况。加速的乳酸产生与已知呼吸链复合物 IV 抑制剂叠氮化物的产生不具有加和性,并且在甲醛暴露 1.5 小时后去除甲醛后仍然存在。这些数据表明,培养的星形胶质细胞能够有效地将甲醛氧化为甲酸盐,随后增强糖酵解通量,这很可能是通过抑制线粒体呼吸实现的。

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