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开发一种基于细胞的高通量荧光素酶酶片段互补分析方法以鉴定核因子E2相关转录因子2激活剂。

Development of a cell-based high throughput luciferase enzyme fragment complementation assay to identify nuclear-factor-e2-related transcription factor 2 activators.

作者信息

Xie Wensheng, Pao Christina, Graham Taylor, Dul Ed, Lu Quinn, Sweitzer Thomas D, Ames Robert S, Li Hu

机构信息

Department of Biological Reagents and Assay Development, Platform Technology and Science, GlaxoSmithKline Pharmaceuticals, Collegeville, Pennsylvania 19426, USA.

出版信息

Assay Drug Dev Technol. 2012 Dec;10(6):514-24. doi: 10.1089/adt.2011.436. Epub 2012 May 10.

DOI:10.1089/adt.2011.436
PMID:22574653
Abstract

Nuclear-factor-E2-related transcription factor 2 (Nrf2) regulates a large panel of Phase II genes and plays an important role in cell survival. Nrf2 activation has been shown as preventing cigarette smoke-induced alveolar enlargement in mice. Therefore, activation of the Nrf2 protein by small-molecule activators represents an attractive therapeutic strategy that is used for chronic obstructive pulmonary disease. In this article, we describe a cell-based luciferase enzyme fragment complementation assay that identifies Nrf2 activators. This assay is based on the interaction of Nrf2 with its nuclear partner MafK or runt-related transcription factor 2 (RunX2) and is dependent on the reconstitution of a "split" luciferase. Firefly luciferase is split into two fragments, which are genetically fused to Nrf2 and MafK or RunX2, respectively. BacMam technology was used to deliver the fusion constructs into cells for expression of the tagged proteins. When the BacMam-transduced cells were treated with Nrf2 activators, the Nrf2 protein was stabilized and translocated into the nucleus where it interacted with MafK or RunX2. The interaction of Nrf2 and MafK or RunX2 brought together the two luciferase fragments that form an active luciferase. The assay was developed in a 384-well format and was optimized by titrating the BacMam concentration, transduction time, cell density, and fetal bovine serum concentration. It was further validated with known Nrf2 activators. Our data show that this assay is robust, sensitive, and amenable to high throughput screening of a large compound collection for the identification of novel Nrf2 activators.

摘要

核因子E2相关转录因子2(Nrf2)调节大量II期基因,并在细胞存活中发挥重要作用。Nrf2激活已被证明可预防香烟烟雾诱导的小鼠肺泡增大。因此,通过小分子激活剂激活Nrf2蛋白代表了一种有吸引力的治疗策略,可用于慢性阻塞性肺疾病。在本文中,我们描述了一种基于细胞的荧光素酶片段互补测定法,用于鉴定Nrf2激活剂。该测定法基于Nrf2与其核伴侣MafK或 runt相关转录因子2(RunX2)的相互作用,并依赖于“分裂”荧光素酶的重组。萤火虫荧光素酶被分成两个片段,分别与Nrf2和MafK或RunX2进行基因融合。使用杆状病毒表达载体技术将融合构建体导入细胞中以表达标记蛋白。当用Nrf2激活剂处理杆状病毒转导的细胞时,Nrf2蛋白被稳定并转运到细胞核中,在那里它与MafK或RunX2相互作用。Nrf2与MafK或RunX2的相互作用使两个荧光素酶片段聚集在一起,形成活性荧光素酶。该测定法以384孔板形式开发,并通过滴定杆状病毒表达载体浓度、转导时间、细胞密度和胎牛血清浓度进行了优化。用已知的Nrf2激活剂进一步验证。我们的数据表明,该测定法稳健、灵敏,适用于对大量化合物库进行高通量筛选,以鉴定新型Nrf2激活剂。

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