Pannexin-1 channels show distinct morphology and no gap junction characteristics in mammalian cells

被引:0
|
作者
Anja Beckmann
Alexander Grissmer
Elmar Krause
Thomas Tschernig
Carola Meier
机构
[1] Saarland University,Department of Anatomy and Cell Biology
[2] Saarland University,Department of Physiology
来源
Cell and Tissue Research | 2016年 / 363卷
关键词
Gap junction; Pannexin; Electron microscopy; Freeze-fracture replica immunolabeling; FRIL;
D O I
暂无
中图分类号
学科分类号
摘要
Pannexins (Panx) are proteins with a similar membrane topology to connexins, the integral membrane protein of gap junctions. Panx1 channels are generally of major importance in a large number of system and cellular processes and their function has been thoroughly characterized. In contrast, little is known about channel structure and subcellular distribution. We therefore determine the subcellular localization of Panx1 channels in cultured cells and aim at the identification of channel morphology in vitro. Using freeze-fracture replica immunolabeling on EYFP-Panx1-overexpressing HEK 293 cells, large particles were identified in plasma membranes, which were immunogold-labeled using either GFP or Panx1 antibodies. There was no labeling or particles in the nuclear membranes of these cells, pointing to plasma membrane localization of Panx1-EYFP channels. The assembly of particles was irregular, this being in contrast to the regular pattern of gap junctions. The fact that no counterparts were identified on apposing cells, which would have been indicative of intercellular signaling, supported the idea of Panx1 channels within one membrane. Control cells (transfected with EYFP only, non-transfected) were devoid of both particles and immunogold labeling. Altogether, this study provides the first demonstration of Panx1 channel morphology and assembly in intact cells. The identification of Panx1 channels as large particles within the plasma membrane provides the knowledge required to enable recognition of Panx1 channels in tissues in future studies. Thus, these results open up new avenues for the detailed analysis of the subcellular localization of Panx1 and of its nearest neighbors such as purinergic receptors in vivo.
引用
收藏
页码:751 / 763
页数:12
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