Direct and specific functional evaluation of the Nrf2 and MafG heterodimer by introducing a tethered dimer into small maf-deficient cells

Fumiki Katsuoka, Akihito Otsuki, Mizue Takahashi, Shin Ito, Masayuki Yamamoto

研究成果: Article査読

7 被引用数 (Scopus)

抄録

A group of cytoprotective genes is regulated by heterodimers composed of the cap'n'collar (CNC) family member Nrf2 and one of the small Maf (sMaf) proteins (MafF, MafG, or MafK) through the antioxidant response element (ARE, also referred to as the CNC-sMaf binding element [CsMBE]). Many lines of evidence support this model; however, a direct and specific evaluation of the Nrf2-sMaf heterodimer remains to be executed. To address this issue, we constructed a tethered Nrf2-MafG (T-N2G) heterodimer using a flexible linker peptide. We then introduced the T-N2G construct into cells lacking all three sMaf proteins to specifically evaluate the function of the tethered heterodimer without interference from other endogenous CNC-sMaf heterodimers or sMaf homodimers. In response to an Nrf2 activator, diethyl maleate, the T-N2G protein can widely activate the target genes of Nrf2 but not those of Nrf1, such as proteasome subunit genes. Genome-wide binding analysis showed that the T-N2G protein preferentially bound to the CsMBE motifs in the regulatory regions of the Nrf2 target genes. These results provide direct evidence that the Nrf2-MafG heterodimer acts as a transcriptional activator of Nrf2-dependent genes and show that this assay system will be a powerful tool to specifically examine the function of other CNC-sMaf heterodimers.

本文言語English
論文番号e00273-19
ジャーナルMolecular and cellular biology
39
20
DOI
出版ステータスPublished - 2019 10 1

ASJC Scopus subject areas

  • Molecular Biology
  • Cell Biology

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