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一种基于细胞的高通量缝隙连接通讯检测方法,适用于使用 IncuCyte ZOOM 评估连接蛋白 43-埃兹蛋白相互作用抑制剂。

A Cell-Based High-Throughput Assay for Gap Junction Communication Suitable for Assessing Connexin 43-Ezrin Interaction Disruptors Using IncuCyte ZOOM.

机构信息

1 Centre for Molecular Medicine Norway, Nordic EMBL Partnership, University of Oslo and Oslo University Hospital, Oslo, Norway.

2 Biotechnology Centre, University of Oslo, Oslo, Norway.

出版信息

SLAS Discov. 2017 Jan;22(1):77-85. doi: 10.1177/1087057116669120. Epub 2016 Sep 26.

DOI:10.1177/1087057116669120
PMID:27628689
Abstract

Connexin 43 (Cx43), the predominant gap junction (GJ) protein, directly interacts with the A-kinase-anchoring protein (AKAP) Ezrin in human cytotrophoblasts and a rat liver epithelial cells (IAR20). The Cx43-Ezrin-protein kinase (PKA) complex facilitates Cx43 phosphorylation by PKA, which triggers GJ opening in cytotrophoblasts and IAR20 cells and may be a general mechanism regulating GJ intercellular communication (GJIC). Considering the importance of Cx43 GJs in health and disease, they are considered potential pharmaceutical targets. The Cx43-Ezrin interaction is a protein-protein interaction that opens possibilities for targeting with peptides and small molecules. For this reason, we developed a high-throughput cell-based assay in which GJIC can be assessed and new compounds characterized. We used two pools of IAR20 cells, calcein loaded and unloaded, that were mixed and allowed to attach. Next, GJIC was monitored over time using automated imaging via the IncuCyte imager. The assay was validated using known GJ inhibitors and anchoring peptide disruptors, and we further tested new peptides that interfered with the Cx43-Ezrin binding region and reduced GJIC. Although an AlphaScreen assay can be used to screen for Cx43-Ezrin interaction inhibitors, the cell-based assay described is an ideal secondary screen for promising small-molecule hits to help identify the most potent compounds.

摘要

间隙连接蛋白 43(Cx43)是主要的间隙连接(GJ)蛋白,它直接与 AKAP 锚蛋白(Ezrin)在人绒毛膜滋养层细胞和大鼠肝上皮细胞(IAR20)中相互作用。Cx43-Ezrin-蛋白激酶(PKA)复合物促进 PKA 对 Cx43 的磷酸化,这触发了绒毛膜滋养层细胞和 IAR20 细胞中 GJ 的开放,可能是调节 GJ 细胞间通讯(GJIC)的一般机制。考虑到 Cx43 GJ 在健康和疾病中的重要性,它们被认为是潜在的药物靶点。Cx43-Ezrin 相互作用是一种蛋白质-蛋白质相互作用,为使用肽和小分子进行靶向提供了可能性。出于这个原因,我们开发了一种高通量基于细胞的测定方法,可以评估 GJIC 并对新化合物进行表征。我们使用了两种 IAR20 细胞池,一种是负载钙黄绿素的,另一种是未负载的,将它们混合并让其附着。然后,通过自动成像 IncuCyte 成像仪监测随着时间的推移 GJIC。该测定方法使用已知的 GJ 抑制剂和锚定肽破坏剂进行了验证,我们还进一步测试了新的肽,这些肽干扰了 Cx43-Ezrin 结合区域并降低了 GJIC。虽然 AlphaScreen 测定法可用于筛选 Cx43-Ezrin 相互作用抑制剂,但所描述的基于细胞的测定法是筛选有前途的小分子命中物的理想二级筛选,有助于识别最有效的化合物。

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