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首页> 外文期刊>Journal of Neurochemistry: Offical Journal of the International Society for Neurochemistry >GLAST/EAAT1-induced Glutamine release via SNAT3 in Bergmann glial cells: Evidence of a functional and physical coupling
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GLAST/EAAT1-induced Glutamine release via SNAT3 in Bergmann glial cells: Evidence of a functional and physical coupling

机译:GLAST / EAAT1诱导的Bergmann胶质细胞中通过SNAT3释放的谷氨酰胺:功能和物理耦合的证据

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摘要

Glutamate, the major excitatory transmitter in the vertebrate brain, is removed from the synaptic cleft by a family of sodium-dependent glutamate transporters profusely expressed in glial cells. Once internalized, it is metabolized by glutamine synthetase to glutamine and released to the synaptic space through sodium-dependent neutral amino acid carriers of the N System (SNAT3/slc38a3/SN1, SNAT5/slc38a5/SN2). Glutamine is then taken up by neurons completing the so-called glutamate/glutamine shuttle. Despite of the fact that this coupling was described decades ago, it is only recently that the biochemical framework of this shuttle has begun to be elucidated. Using the established model of cultured cerebellar Bergmann glia cells, we sought to characterize the functional and physical coupling of glutamate uptake and glutamine release. A time-dependent Na+-dependent glutamate/aspartate transporter/EAAT1-induced System N-mediated glutamine release could be demonstrated. Furthermore, D-aspartate, a specific glutamate transporter ligand, was capable of enhancing the co-immunoprecipitation of Na+-dependent glutamate/aspartate transporter and Na+-dependent neutral amino acid transporter 3, whereas glutamine tended to reduce this association. Our results suggest that glial cells surrounding glutamatergic synapses may act as sensors of neuron-derived glutamate through their contribution to the neurotransmitter turnover. A functional and physical coupling of glutamate uptake and glutamine release was characterized using cerebellar Bergmannglia cells. A time-dependent, GLAST-induced System N-mediated glutamine release could be demonstrated and a co-immunoprecipitation of GLAST and SNAT3 is described. Our results suggest that glial cells surrounding glutamatergic synapses may act as sensors of neuron-derived glutamate through their contribution to the turnover of this neurotransmitter.
机译:谷氨酸是脊椎动物大脑中的主要兴奋性递质,它通过在胶质细胞中大量表达的钠依赖性谷氨酸转运蛋白家族从突触间隙中去除。一旦内在化,它就被谷氨酰胺合成酶代谢成谷氨酰胺,并通过N系统的钠依赖性中性氨基酸载体(SNAT3 / slc38a3 / SN1,SNAT5 / slc38a5 / SN2)释放到突触空间。然后,谷氨酰胺被神经元吸收,完成所谓的谷氨酸/谷氨酰胺穿梭。尽管已经在几十年前描述了这种偶联,但是直到最近才才阐明这种穿梭的生物化学框架。使用已建立的培养的小脑Bergmann胶质细胞模型,我们试图表征谷氨酸摄取和谷氨酰胺释放的功能和物理耦合。可以证明时间依赖性的Na +依赖性谷氨酸/天冬氨酸转运蛋白/ EAAT1诱导的系统N介导的谷氨酰胺释放。此外,D-天冬氨酸(一种特定的谷氨酸转运蛋白配体)能够增强Na +依赖性谷氨酸/天冬氨酸转运蛋白和Na +依赖性中性氨基酸转运蛋白3的免疫共沉淀,而谷氨酰胺则倾向于减少这种结合。我们的结果表明,围绕谷氨酸能突触的神经胶质细胞可能通过其对神经递质更新的贡献而充当神经元衍生的谷氨酸的传感器。谷氨酸摄取和谷氨酰胺释放的功能和物理耦合使用小脑Bergmannglia细胞进行了表征。可以证明时间依赖性的GLAST诱导的系统N介导的谷氨酰胺释放,并描述了GLAST和SNAT3的免疫共沉淀。我们的结果表明,围绕谷氨酸能突触的神经胶质细胞可能通过其对这种神经递质的更新的贡献而充当神经元衍生的谷氨酸的传感器。

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