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用于鉴定p53-hDM2蛋白质-蛋白质相互作用干扰物的高内涵筛选生物传感器检测法。

High content screening biosensor assay to identify disruptors of p53-hDM2 protein-protein interactions.

作者信息

Hua Yun, Strock Christopher J, Johnston Paul A

机构信息

Department of Pharmaceutical Sciences, School of Pharmacy, University of Pittsburgh, Room 1014 Salk Hall, 3501 Terrace Street, Pittsburgh, PA, 15261, USA.

出版信息

Methods Mol Biol. 2015;1278:555-65. doi: 10.1007/978-1-4939-2425-7_37.

DOI:10.1007/978-1-4939-2425-7_37
PMID:25859976
Abstract

This chapter describes the implementation of the p53-hDM2 protein-protein interaction (PPI) biosensor (PPIB) HCS assay to identify disruptors of p53-hDM2 PPIs. Recombinant adenovirus expression constructs were generated bearing the individual p53-GFP and hDM2-RFP PPI partners. The N-terminal p53 transactivating domain that contains the binding site for hDM2 is expressed as a GFP fusion protein that is targeted and anchored in the nucleolus of infected cells by a nuclear localization (NLS) sequence. The p53-GFP biosensor is localized to the nucleolus to enhance and facilitate the image acquisition and analysis of the PPIs. The N-terminus of hDM2 encodes the domain for binding to the transactivating domain of p53, and is expressed as a RFP fusion protein that includes both an NLS and a nuclear export sequence (NES). In U-2 OS cells co-infected with both adenovirus constructs, the binding interactions between hDM2 and p53 result in both biosensors becoming co-localized within the nucleolus. Upon disruption of the p53-hDM2 PPIs, the p53-GFP biosensor remains in the nucleolus while the shuttling hDM2-RFP biosensor redistributes into the cytoplasm. p53-hDM2 PPIs are measured by acquiring fluorescent images of cells co-infected with both adenovirus biosensors on an automated HCS imaging platform and using an image analysis algorithm to quantify the relative distribution of the hDM2-RFP shuttling component of the biosensor between the cytoplasm and nuclear regions of compound treated cells.

摘要

本章描述了p53-hDM2蛋白质-蛋白质相互作用(PPI)生物传感器(PPIB)的高内涵筛选(HCS)分析方法的实施过程,以鉴定p53-hDM2 PPI的干扰剂。构建了携带单个p53-GFP和hDM2-RFP PPI伙伴的重组腺病毒表达构建体。包含hDM2结合位点的p53 N端反式激活结构域表达为GFP融合蛋白,该蛋白通过核定位(NLS)序列靶向并锚定在受感染细胞的核仁中。p53-GFP生物传感器定位于核仁,以增强和促进PPI的图像采集和分析。hDM2的N端编码与p53反式激活结构域结合的结构域,并表达为RFP融合蛋白,该蛋白同时包含NLS和核输出序列(NES)。在同时感染两种腺病毒构建体的U-2 OS细胞中,hDM2和p53之间的结合相互作用导致两种生物传感器在核仁内共定位。当p53-hDM2 PPI被破坏时,p53-GFP生物传感器保留在核仁中,而穿梭的hDM2-RFP生物传感器重新分布到细胞质中。通过在自动化HCS成像平台上获取同时感染两种腺病毒生物传感器的细胞的荧光图像,并使用图像分析算法来量化化合物处理细胞的细胞质和细胞核区域之间生物传感器的hDM2-RFP穿梭成分的相对分布,来测量p53-hDM2 PPI。

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