BioTechniques (May 2005)

Improved T-DNA vector for tagging plant promoters via high-throughput luciferase screening

  • Serge Remy,
  • Els Thiry Bertcoemans,
  • Saskia Windelinckx,
  • Rony Swennen,
  • László Sági

DOI
https://doi.org/10.2144/05385RR01
Journal volume & issue
Vol. 38, no. 5
pp. 763 – 770

Abstract

Read online

Transferred DNA (T-DNA) tagging is a powerful tool for tagging and in planta characterization of plant genes on a genome-wide scale. An improved promoter tagging vector is described here, which contains the codon-optimized luciferase (luc+) reporter gene 31 bpfrom the right border of the T-DNA. Compared to the wild-type luciferase gene, this construct provides significantly increased reporter gene expression and a 40 times higher tagging frequency. The utility of the construct is demonstrated in banana, a tropical monocot species, by screening embryogenic cell colonies and regenerated plants with an ultrasensitive charged-coupled device (CCD) camera. The improved vector resulted in a luciferase activation frequency of 2.5% in 19,000 cell colonies screened. Detailed molecular analysis of flanking DNA sequences in a tagged line revealed insertion of the luciferase tag in a novel gene with near-constitutive expression.