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连接蛋白类型和荧光蛋白融合标签决定间隙连接斑块的结构稳定性。

Connexin Type and Fluorescent Protein Fusion Tag Determine Structural Stability of Gap Junction Plaques.

作者信息

Stout Randy F, Snapp Erik Lee, Spray David C

机构信息

From the Dominick P. Purpura Department of Neuroscience and.

the Department of Anatomy and Structural Biology, Albert Einstein College of Medicine, Bronx, New York 10461.

出版信息

J Biol Chem. 2015 Sep 25;290(39):23497-514. doi: 10.1074/jbc.M115.659979. Epub 2015 Aug 11.

Abstract

Gap junctions (GJs) are made up of plaques of laterally clustered intercellular channels and the membranes in which the channels are embedded. Arrangement of channels within a plaque determines subcellular distribution of connexin binding partners and sites of intercellular signaling. Here, we report the discovery that some connexin types form plaque structures with strikingly different degrees of fluidity in the arrangement of the GJ channel subcomponents of the GJ plaque. We uncovered this property of GJs by applying fluorescence recovery after photobleaching to GJs formed from connexins fused with fluorescent protein tags. We found that connexin 26 (Cx26) and Cx30 GJs readily diffuse within the plaque structures, whereas Cx43 GJs remain persistently immobile for more than 2 min after bleaching. The cytoplasmic C terminus of Cx43 was required for stability of Cx43 plaque arrangement. We provide evidence that these qualitative differences in GJ arrangement stability reflect endogenous characteristics, with the caveat that the sizes of the GJs examined were necessarily large for these measurements. We also uncovered an unrecognized effect of non-monomerized fluorescent protein on the dynamically arranged GJs and the organization of plaques composed of multiple connexin types. Together, these findings redefine our understanding of the GJ plaque structure and should be considered in future studies using fluorescent protein tags to probe dynamics of highly ordered protein complexes.

摘要

间隙连接(GJs)由横向聚集的细胞间通道斑块以及嵌入通道的膜组成。斑块内通道的排列决定了连接蛋白结合伙伴的亚细胞分布和细胞间信号传导位点。在此,我们报告发现某些连接蛋白类型形成的斑块结构,其间隙连接斑块的间隙连接(GJ)通道亚组分排列具有显著不同程度的流动性。我们通过对与荧光蛋白标签融合的连接蛋白形成的间隙连接应用光漂白后的荧光恢复来揭示间隙连接的这一特性。我们发现连接蛋白26(Cx26)和Cx30间隙连接在斑块结构内易于扩散,而Cx43间隙连接在漂白后超过2分钟仍持续保持不动。Cx43的细胞质C末端是Cx43斑块排列稳定性所必需的。我们提供的证据表明,间隙连接排列稳定性的这些定性差异反映了内源性特征,但需注意的是,对于这些测量而言,所检测的间隙连接尺寸必然较大。我们还发现了未单体化的荧光蛋白对动态排列的间隙连接以及由多种连接蛋白类型组成的斑块组织的一种未被认识到的影响。总之,这些发现重新定义了我们对间隙连接斑块结构的理解,并且在未来使用荧光蛋白标签探测高度有序蛋白质复合物动态的研究中应予以考虑。

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