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在解离的小鼠大脑皮层共培养系统中证明γ-氨基丁酸(GABA)生物合成前体的神经元-神经胶质细胞转移

Demonstration of neuron-glia transfer of precursors for GABA biosynthesis in a co-culture system of dissociated mouse cerebral cortex.

作者信息

Leke Renata, Bak Lasse K, Schousboe Arne, Waagepetersen Helle S

机构信息

Department of Pharmacology and Pharmacotherapy, Faculty of Pharmaceutical Sciences, University of Copenhagen, Universitetsparken 2, 2100, Copenhagen, Denmark.

出版信息

Neurochem Res. 2008 Dec;33(12):2629-35. doi: 10.1007/s11064-008-9814-6. Epub 2008 Aug 16.

Abstract

Co-cultures of neurons and astrocytes were prepared from dissociated embryonic mouse cerebral cortex and cultured for 7 days. To investigate if these cultures may serve as a functional model system to study neuron-glia interaction with regard to GABA biosynthesis, the cells were incubated either in media containing [U-(13)C]glutamine (0.1, 0.3 and 0.5 mM) or 1 mM acetate plus 2.5 mM glucose plus 1 mM lactate. In the latter case one of the 3 substrates was uniformly (13)C labeled. Cellular contents and (13)C labeling of glutamate, GABA, aspartate and glutamine were determined in the cells after an incubation period of 2.5 h. The GABA biosynthetic machinery exhibited the expected complexity with regard to metabolic compartmentation and involvement of TCA cycle activity as seen in other culture systems containing GABAergic neurons. Metabolism of acetate clearly demonstrated glial synthesis of glutamine and its transfer to the neuronal compartment. It is concluded that this co-culture system serves as a reliable model in which functional and pharmacological aspects of GABA biosynthesis can be investigated.

摘要

从解离的胚胎小鼠大脑皮层制备神经元和星形胶质细胞的共培养物,并培养7天。为了研究这些培养物是否可作为一个功能模型系统,用于研究神经元 - 胶质细胞在GABA生物合成方面的相互作用,将细胞分别在含有[U-(13)C]谷氨酰胺(0.1、0.3和0.5 mM)或1 mM乙酸盐加2.5 mM葡萄糖加1 mM乳酸盐的培养基中孵育。在后一种情况下,三种底物之一用(13)C均匀标记。在孵育2.5小时后,测定细胞中谷氨酸、GABA、天冬氨酸和谷氨酰胺的细胞含量及(13)C标记情况。与其他含有GABA能神经元的培养系统一样,GABA生物合成机制在代谢区室化和三羧酸循环活性参与方面表现出预期的复杂性。乙酸盐的代谢清楚地表明了星形胶质细胞对谷氨酰胺的合成及其向神经元区室的转运。得出的结论是,这种共培养系统是一个可靠的模型,可用于研究GABA生物合成的功能和药理学方面。

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