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Cloning and characterization of a gene encoding ABP57, a soluble auxin-binding protein

  • Lee, Keunpyo (National Academy of Agricultural Science, Rural Development Administration) ;
  • Kim, Myung-Il (Department of Agricultural Biotechnology, Seoul National University) ;
  • Kwon, Yu-Jihn (Hazardous Substance Analysis Division, Korea Food and Drug Administration) ;
  • Kim, Minkyun (Department of Agricultural Biotechnology, Seoul National University) ;
  • Kim, Yong-Sam (Daejeon-KRIBB-FHCRC Research Cooperation Center, KRIBB) ;
  • Kim, Donghern (National Academy of Agricultural Science, Rural Development Administration)
  • Received : 2009.06.15
  • Accepted : 2009.06.24
  • Published : 2009.10.31

Abstract

Auxin-binding protein 57 ($ABP_{57}$), a soluble auxin-binding protein, acts as a receptor to activate plasma membrane (PM) $H^+-ATPase$. Here, we report the cloning of abp57 and the biochemical characterization of its protein expressed in E. coli. The analysis of internal amino acid sequences of $ABP_{57}$ purified from rice shoots enabled us to search for the corresponding gene in protein DB of NCBI. Further BLAST analysis showed that rice has four abp57-like genes and maize has at least one homolog. Interestingly, Arabidopsis seems to have no homolog. Recombinant $ABP_{57}$ expressed in E. coli caused the activation of PM $H^+-ATPase$ regardless of the existence of IAA. Scatchard analysis showed that the recombinant protein has relatively low affinity to IAA as compared to natural $ABP_{57}$. These results collectively support the notion that the cloned gene is responsible for $ABP_{57}$.

Keywords

Acknowledgement

Supported by : National Academy of Agricultural Science, Rural Development Administration

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