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      Synthetic gene involving azobenzene-tethered T7 promoter for the photocontrol of gene expression by visible light.

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          Abstract

          In the present study, we demonstrate photoregulation of gene expression in a cell-free translation system from a T7 promoter containing two azobenzene derivatives at specific positions. As photoswitches, we prepared azobenzene-4'-carboxlyic acid (Azo) and 2,6-dimethylazobenzene-4'-carboxylic acid (DM-Azo), which were isomerized from trans to cis upon irradiation with UV light (λ < 370 nm), and 4-methylthioazobenzene-4'-carboxylic acid (S-Azo) and 2,6-dimethyl-4-(methylthio)azobenzene-4'-carobxylic acid (S-DM-Azo), which were cis-isomerized by irradiation with 400 nm visible light. Expression of green fluorescent protein from a promoter modified with S-Azo or S-DM-Azo could be induced by harmless visible light whereas that from a promoter modified with Azo or DM-Azo was induced only by UV light (340-360 nm). Thus, efficient photoregulation of green fluorescent protein production was achieved in a cell-free translation system with visible light without photodamage.

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          Author and article information

          Journal
          ACS Synth Biol
          ACS synthetic biology
          American Chemical Society (ACS)
          2161-5063
          2161-5063
          Apr 17 2015
          : 4
          : 4
          Affiliations
          [1 ] §School of Food Science and Engineering, Ocean University of China, Yushan-lu 5, Shinanqu, Qingdao 266003, China.
          Article
          10.1021/sb5001092
          25144622
          759e6311-33a4-40cb-82f2-69e53979c6b2
          History

          azobenzene,d-threoninol scaffold,gene expression,photoactivated,transcription,visible light

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