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首页> 外文期刊>Neuropeptides: An International Journal >Constitutive and ligand-induced internalization of EGFP-tagged galanin R2 and Rl receptors in PC12 cells.
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Constitutive and ligand-induced internalization of EGFP-tagged galanin R2 and Rl receptors in PC12 cells.

机译:PC12细胞中EGFP标签的甘丙肽R2和R1受体的组成性和配体诱导的内在化。

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摘要

In the present experiments trafficking of the galanin R1-(GALR1) and, in particular, the galanin R2 receptor (GALR2) was studied after fusion with enhanced green fluorescent protein (GALR1-EGFP and GALR2-EGFP) and transfection into PC12 cells. Both fusion proteins were predominantly localized on the plasma membrane and internalized in a dose dependent manner after incubation with galanin. Preincubation with M35 or M40 did not prevent galanin-induced internalization of GALR1-EGFP or GALR2-EGFP. However, AR-M1896, a selective GALR2 agonist, caused GALR2, but not GALR1 internalization. Hyperosmotic sucrose inhibited internalization of GALR2-EGFP. After co-incubation with galanin, GALR2-EGFP was co-localized with internalized Texas Red transferrin, a marker of the clathrin endocytic pathway. Experiments with protein synthesis inhibition and Texas Red transferrin suggest that GALR2 is constitutively internalized. Studies in progress will show if this is the case also for GALR1.
机译:在本实验中,在与增强的绿色荧光蛋白(GALR1-EGFP和GALR2-EGFP)融合并转染到PC12细胞中后,研究了甘丙肽R1-(GALR1),特别是甘丙肽R2受体(GALR2)的运输。与甘丙肽温育后,两种融合蛋白主要定位在质膜上,并以剂量​​依赖性方式内在化。与M35或M40预孵育不能阻止甘丙肽诱导的GALR1-EGFP或GALR2-EGFP的内在化。但是,选择性GALR2激动剂AR-M1896引起了GALR2,但没有引起GALR1内在化。高渗蔗糖抑制GALR2-EGFP的内在化。与甘丙肽共同孵育后,GALR2-EGFP与内在的德克萨斯红转铁蛋白(网格蛋白内吞途径的标志物)共定位。蛋白质合成抑制和德克萨斯红转铁蛋白的实验表明,GALR2是组成型内在化的。正在进行的研究将显示GALR1是否也是如此。

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