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G蛋白偶联生长抑素受体sst2在人胶质瘤细胞中的信号转导拓扑结构。

Topology of the signal transduction of the G protein-coupled somatostatin receptor sst2 in human glioma cells.

作者信息

Mentlein R, Held-Feindt J, Krisch B

机构信息

Anatomisches Institut der Universität Kiel, Germany.

出版信息

Cell Tissue Res. 2001 Jan;303(1):27-34. doi: 10.1007/s004410000302.

DOI:10.1007/s004410000302
PMID:11236002
Abstract

By a dual approach, using electron microscopy and biochemical techniques, we investigated the topology of the somatostatin receptor sst2 with its inhibitory G protein Gialpha after ligand-induced stimulation and internalization in human glioma cells. On intact cells, the sst2 was labeled at 8 degrees C by an antibody directed to its extracellular sequence followed by a 15-nm gold-labeled secondary antibody. In the presence of the ligand, internalization was induced by exposure to 37 degrees C for 5-10 min. Then, cells were either fixed for immunoelectron-microscopic analysis or homogenized for density gradient separation. After post-embedding staining of the sst2-labeled sections with anti-Gialpha1- 3 or anti-caveolin, a co-localization of sst2, Gialpha and caveolin was detected in endosomal vesicles after 5 min of internalization, but not after 10 min. Furthermore, the gold-labeled organelles containing the internalised receptor were separated from the non-labeled ones on sucrose gradients (density shift separation) and analyzed by Western blotting. Also here, in fractions with higher densities, sst2 could be costained with Gialpha and caveolin after 5 min. From these congruent results from both methods, it can be concluded that, in human glioma cells, the receptor sst2 (1) is internalised in caveolin-positive vesicles and (2) is neighboured to its Gialpha proteins at the plasma membrane and early endosomes.

摘要

通过电子显微镜和生化技术相结合的方法,我们研究了在人胶质瘤细胞中,生长抑素受体sst2及其抑制性G蛋白Gialpha在配体诱导的刺激和内化后的拓扑结构。在完整细胞上,在8摄氏度时,用针对其细胞外序列的抗体标记sst2,随后用15纳米金标记的二抗进行标记。在存在配体的情况下,通过在37摄氏度下暴露5至10分钟诱导内化。然后,将细胞固定用于免疫电子显微镜分析,或匀浆用于密度梯度分离。在用抗Gialpha1 - 3或抗小窝蛋白对sst2标记的切片进行包埋后染色后,在内化5分钟后在内体小泡中检测到sst2、Gialpha和小窝蛋白的共定位,但10分钟后未检测到。此外,在蔗糖梯度上(密度移位分离)将含有内化受体的金标记细胞器与未标记的细胞器分离,并通过蛋白质免疫印迹法进行分析。同样在这里,在较高密度的组分中,5分钟后sst2可以与Gialpha和小窝蛋白共染色。从这两种方法得到的一致结果可以得出结论,在人胶质瘤细胞中,受体sst2(1)在内化到小窝蛋白阳性小泡中,(2)在质膜和早期内体中与其Gialpha蛋白相邻。

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