Gene Trapping with Firefly Luciferase in Arabidopsis. Tagging of Stress-Responsive Genes

Author:

Alvarado Martha C.1,Zsigmond Laura M.1,Kovács Izabella1,Cséplö Ágnes1,Koncz Csaba1,Szabados László M.1

Affiliation:

1. Institute of Plant Biology, Biological Research Center, Temesvári krt. 62, 6726-Szeged, Hungary (M.C.A., L.Z., I.K., A.C., L.M.S.); and Max-Planck-Institut für Züchtungsforschung, Carl-von-Linné-Weg 10, D-50829-Köln, Germany (C.K.)

Abstract

Abstract To monitor the expression of T-DNA-tagged plant genes in vivo, a collection of 20,261 transgenic lines of Arabidopsis (Columbia-0) were generated with the promoter trap vector pTluc, which carries a promoterless firefly luc (luciferase) reporter gene linked to the right T-DNA border. By detection of bioluminescence in 3-week-old seedlings, 753 lines were identified showing constitutive, organ-specific, and stress-responsive luciferase expression patterns. To facilitate the identification of well-defined luciferase expression patterns, a pooled seed stock was established. Several lines showed sugar, salt, and abscisic acid (ABA)-inducible luciferase activity. Segregation analysis of 215 promoter trap lines indicated that about 50% of plants contained single insertions, whereas 40% carried two and 10% carried three or more T-DNA tags. Sequencing the T-DNA insert junctions isolated from 17 luciferase-expressing lines identified T-DNA tags in 5′- and 3′-transcribed domains and translational gene fusions generated by T-DNA insertions in exons and introns of Arabidopsis genes. Tissue specific expression of eight wild-type Arabidopsis genes was confirmed to be similar to the luminescence patterns observed in the corresponding luciferase-tagged lines. Here, we describe the characterization of a transcriptional luc reporter gene fusion with the WBC-type ABC transporter gene At1g17840. Expression of wild-type and luciferase-tagged At1g17840 alleles revealed similar induction by salt, glucose, and ABA treatments and gibberellin-mediated down-regulation of ABA-induced expression. These results illustrate that luciferase gene traps are well suited for monitoring the expression of stress-responsive Arabidopsis genes in vivo.

Publisher

Oxford University Press (OUP)

Subject

Plant Science,Genetics,Physiology

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