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Keap1通过与氨基末端Neh2结构域结合,抑制Nrf2对抗氧化反应元件的核激活。

Keap1 represses nuclear activation of antioxidant responsive elements by Nrf2 through binding to the amino-terminal Neh2 domain.

作者信息

Itoh K, Wakabayashi N, Katoh Y, Ishii T, Igarashi K, Engel J D, Yamamoto M

机构信息

Center for Tsukuba Advanced Research Alliance and Institute of Basic Medical Sciences, University of Tsukuba, Tsukuba 305-8577, Japan.

出版信息

Genes Dev. 1999 Jan 1;13(1):76-86. doi: 10.1101/gad.13.1.76.

Abstract

Transcription factor Nrf2 is essential for the antioxidant responsive element (ARE)-mediated induction of phase II detoxifying and oxidative stress enzyme genes. Detailed analysis of differential Nrf2 activity displayed in transfected cell lines ultimately led to the identification of a new protein, which we named Keap1, that suppresses Nrf2 transcriptional activity by specific binding to its evolutionarily conserved amino-terminal regulatory domain. The closest homolog of Keap1 is a Drosophila actin-binding protein called Kelch, implying that Keap1 might be a Nrf2 cytoplasmic effector. We then showed that electrophilic agents antagonize Keap1 inhibition of Nrf2 activity in vivo, allowing Nrf2 to traverse from the cytoplasm to the nucleus and potentiate the ARE response. We postulate that Keap1 and Nrf2 constitute a crucial cellular sensor for oxidative stress, and together mediate a key step in the signaling pathway that leads to transcriptional activation by this novel Nrf2 nuclear shuttling mechanism. The activation of Nrf2 leads in turn to the induction of phase II enzyme and antioxidative stress genes in response to electrophiles and reactive oxygen species.

摘要

转录因子Nrf2对于抗氧化反应元件(ARE)介导的II期解毒和氧化应激酶基因的诱导至关重要。对转染细胞系中显示的Nrf2差异活性进行详细分析,最终导致鉴定出一种新蛋白,我们将其命名为Keap1,它通过特异性结合其进化保守的氨基末端调节域来抑制Nrf2转录活性。Keap1最接近的同源物是一种名为Kelch的果蝇肌动蛋白结合蛋白,这意味着Keap1可能是Nrf2的细胞质效应物。然后我们表明,亲电试剂在体内拮抗Keap1对Nrf2活性的抑制,使Nrf2从细胞质转移到细胞核并增强ARE反应。我们推测Keap1和Nrf2构成了氧化应激的关键细胞传感器,并共同介导了信号通路中的一个关键步骤,该信号通路通过这种新型的Nrf2核穿梭机制导致转录激活。Nrf2的激活进而导致II期酶和抗氧化应激基因的诱导,以响应亲电试剂和活性氧。

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