Plant Enzymes but Not Agrobacterium VirD2 Mediate T-DNA Ligation In Vitro

Author:

Ziemienowicz Alicja12,Tinland Bruno1,Bryant John3,Gloeckler Veronique1,Hohn Barbara1

Affiliation:

1. Friedrich Miescher-Institut, CH-4002 Basel, Switzerland1;

2. Plant Pathology Laboratory, Department of Biotechnology, Intercollegiate Faculty of Biotechnology, University of Gdansk, Gdansk, Poland2; and

3. Department of Biological Sciences, University of Exeter, EX4 4QG Exeter, United Kingdom3

Abstract

ABSTRACT Agrobacterium tumefaciens , a gram-negative soil bacterium, transfers DNA to many plant species. In the plant cell, the transferred DNA (T-DNA) is integrated into the genome. An in vitro ligation-integration assay has been designed to investigate the mechanism of T-DNA ligation and the factors involved in this process. The VirD2 protein, which is produced in Agrobacterium and is covalently attached to T-DNA, did not, under our assay conditions, ligate T-DNA to a model target sequence in vitro. We tested whether plant extracts could ligate T-DNA to target oligonucleotides in our test system. The in vitro ligation-integration reaction did indeed take place in the presence of plant extracts. This reaction was inhibited by dTTP, indicating involvement of a plant DNA ligase. We found that prokaryotic DNA ligases could substitute for plant extracts in this reaction. Ligation of the VirD2-bound oligonucleotide to the target sequence mediated by T4 DNA ligase was less efficient than ligation of a free oligonucleotide to the target. T-DNA ligation mediated by a plant enzyme(s) or T4 DNA ligase requires ATP.

Publisher

American Society for Microbiology

Subject

Cell Biology,Molecular Biology

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