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Alternative Splicing of the C-Terminal Domain Regulates Cell Surface Expression of the NMDA Receptor NR1 Subunit

机译:C末端域的选择性剪接调节NMDA受体NR1亚基的细胞表面表达。

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摘要

Subcellular localization of the NMDA receptor NR1 splice forms was studied by expressing individual splice variants and their epitope-tagged derivatives in mouse fibroblasts and in hippocampal neurons. When NR1 splice variants were expressed in fibroblasts, the amount of NR1 molecules expressed on the cell surface varied among forms with different C-terminal cytoplasmic domains. The splice forms with the longest C-terminal cytoplasmic tail (NR1–1a and NR1-1b) showed the lowest amount of cell surface expression, and the splice forms with the shortest C-terminal cytoplasmic tail (NR1–4a and NR1-4b) showed the highest cell surface expression. Cell surface expression of NR1 was enhanced by the coexpression of the NR2 subunit. We measured the glutamate-induced increase of calcium concentration in fibroblasts expressing one of the NR1 splice forms and the NR2B subunit. The increase of calcium concentration after glutamate application had a positive correlation with the amount of NR1 splice forms expressed on the cell surface. When epitope-tagged NR1 splice variants were expressed in primary hippocampal neurons using recombinant adenoviruses, we also observed the differential expression on the cell surface between splice variants. These results suggest that the splicing of the C-terminal domain of the NR1 subunit regulates the cell surface expression of the functional NMDA receptors.
机译:通过在小鼠成纤维细胞和海马神经元中表达单个剪接变体及其表位标记的衍生物,研究了NMDA受体NR1剪接形式的亚细胞定位。当NR1剪接变体在成纤维细胞中表达时,在细胞表面表达的NR1分子的数量在具有不同C端胞质域的形式之间变化。 C端胞质尾巴最长的剪接形式(NR1-1a和NR1-1b)显示最低的细胞表面表达,而C端胞质尾巴最短的剪接形式(NR1-4a和NR1-4b)显示最高的细胞表面表达。 NR2亚基的共表达增强了NR1的细胞表面表达。我们测量了表达NR1剪接形式和NR2B亚基之一的成纤维细胞中谷氨酸诱导的钙浓度增加。谷氨酸施用后钙浓度的增加与细胞表面表达的NR1剪接形式的数量呈正相关。当使用重组腺病毒在原代海马神经元中表达表位标记的NR1剪接变体时,我们还观察到了剪接变体之间在细胞表面的差异表达。这些结果表明,NR1亚基的C端域的剪接调节功能性NMDA受体的细胞表面表达。

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