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SNAT2氨基酸转运体受新皮质神经元中SLC6γ-氨基丁酸转运体亚家族氨基酸的调节,可能在为谷氨酸能传递提供谷氨酰胺方面不起作用。

SNAT2 amino acid transporter is regulated by amino acids of the SLC6 gamma-aminobutyric acid transporter subfamily in neocortical neurons and may play no role in delivering glutamine for glutamatergic transmission.

作者信息

Grewal Sukhjeevan, Defamie Norah, Zhang Xiong, De Gois Stéphanie, Shawki Ali, Mackenzie Bryan, Chen Chu, Varoqui Hélène, Erickson Jeffrey D

机构信息

Neuroscience Center, Louisiana State University Health Science Center, New Orleans, Louisiana 70112, USA.

出版信息

J Biol Chem. 2009 Apr 24;284(17):11224-36. doi: 10.1074/jbc.M806470200. Epub 2009 Feb 24.

Abstract

System A transporters SNAT1 and SNAT2 mediate uptake of neutral alpha-amino acids (e.g. glutamine, alanine, and proline) and are expressed in central neurons. We tested the hypothesis that SNAT2 is required to support neurotransmitter glutamate synthesis by examining spontaneous excitatory activity after inducing or repressing SNAT2 expression for prolonged periods. We stimulated de novo synthesis of SNAT2 mRNA and increased SNAT2 mRNA stability and total SNAT2 protein and functional activity, whereas SNAT1 expression was unaffected. Increased endogenous SNAT2 expression did not affect spontaneous excitatory action-potential frequency over control. Long term glutamine exposure strongly repressed SNAT2 expression but increased excitatory action-potential frequency. Quantal size was not altered following SNAT2 induction or repression. These results suggest that spontaneous glutamatergic transmission in pyramidal neurons does not rely on SNAT2. To our surprise, repression of SNAT2 activity was not limited to System A substrates. Taurine, gamma-aminobutyric acid, and beta-alanine (substrates of the SLC6 gamma-aminobutyric acid transporter family) repressed SNAT2 expression more potently (10x) than did System A substrates; however, the responses to System A substrates were more rapid. Since ATF4 (activating transcription factor 4) and CCAAT/enhancer-binding protein are known to bind to an amino acid response element within the SNAT2 promoter and mediate induction of SNAT2 in peripheral cell lines, we tested whether either factor was similarly induced by amino acid deprivation in neurons. We found that glutamine and taurine repressed the induction of both transcription factors. Our data revealed that SNAT2 expression is constitutively low in neurons under physiological conditions but potently induced, together with the taurine transporter TauT, in response to depletion of neutral amino acids.

摘要

A系统转运蛋白SNAT1和SNAT2介导中性α-氨基酸(如谷氨酰胺、丙氨酸和脯氨酸)的摄取,并在中枢神经元中表达。我们通过长时间诱导或抑制SNAT2表达后检测自发兴奋性活动,来检验SNAT2是支持神经递质谷氨酸合成所必需的这一假设。我们刺激了SNAT2 mRNA的从头合成,提高了SNAT2 mRNA的稳定性以及总SNAT2蛋白和功能活性,而SNAT1的表达未受影响。内源性SNAT2表达增加并未改变对照条件下的自发兴奋性动作电位频率。长期谷氨酰胺暴露强烈抑制了SNAT2表达,但增加了兴奋性动作电位频率。SNAT2诱导或抑制后量子大小未改变。这些结果表明,锥体神经元中的自发谷氨酸能传递不依赖于SNAT2。令我们惊讶的是,SNAT2活性的抑制并不局限于A系统底物。牛磺酸、γ-氨基丁酸和β-丙氨酸(SLC6γ-氨基丁酸转运蛋白家族的底物)比A系统底物更有效地(10倍)抑制SNAT2表达;然而,对A系统底物的反应更快。由于已知激活转录因子4(ATF4)和CCAAT/增强子结合蛋白可结合SNAT2启动子内的氨基酸反应元件并介导外周细胞系中SNAT2的诱导,我们测试了在神经元中氨基酸剥夺是否同样诱导这两种因子。我们发现谷氨酰胺和牛磺酸抑制了这两种转录因子的诱导。我们的数据显示,在生理条件下,神经元中SNAT2的表达本底较低,但在中性氨基酸耗竭时,与牛磺酸转运蛋白TauT一起被强烈诱导。

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