Oct 12, 2005
Research Projects
Production of marker-gene-free barley plants by means of outcrossing after co-transformation
(2001 – 2004) Max Planck Institute (MPI) for Plant Breeding Research, Cologne
Topic
The purpose of the research was to develop a system whereby target and marker genes are incorporated into the plant genome independently of each other by means of agrobacterium-mediated transformation (co-transformation).
- A suitable co-transformation system is a precondition for eliminating the marker gene in the progeny of the transformed plant by means fo segregation.
- A further aim is to prevent unwanted DNA from being transferred during agrobacterium-mediated transformation.
Further information on methods:
Summary
Using comparative investigations, it was possible to demonstrate in this project that plants can be produced without selection markers in a very simple way by means of outcrossing followed by PCR analysis.
Segregation can be achieved in a very simple way by carrying out the co-transformation with two agrobacterium strains, each with one plasmid with the target gene or marker gene. The special feature of this approach is that one can use the same strain of bacteria with an optimum selection marker for every transformation – even with different target genes. This removes the need for costly cloning of the plasmids. The system is utilizable immediately.
Experiment description
Transgenic barley plants in the greenhouse
Representation of the tissue culture stages to obtain a shoot
Work was carried out on the development of suitable binary vectors. At the same time, conditions were established under which these vectors can also be used for transformation of monocotyledons.
Two co-transformation approaches were compared: one agrobacterium strain with one plasmid bearing two T-DNAs, and two agrobacterium strains each with one plasmid (one with the target gene and one with the selection gene).
The transgenic plants were then ripened in the greenhouse for segregation analysis (self-fertilization, cross-pollination). Molecular biological tests were carried out on the next generation to establish how frequently transgenic plants occur without a selection gene. The plants were also subjected to molecular biological analyses (PCR, Southern hybridisation).
Embryo Rescue was used with the aim of accelerating the breeding of the next generation.
Results
Barley of the Golden Promise variety was transformed using both co-transformation methods. More than one hundred transgenic plants were tested. Both methods resulted in segregation, i.e. the PCR method found plants without a selection gene but with the target gene.
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Grant
Bundesministerium für Bildung und Forschung
Förderkennzeichen
0312627 L
Project
Original title
Markergen-Eliminierung basierend auf unabhängiger Cointegration nach agrobacterium tumefaciens- vermittelter Transformation
Contact
Prof. Dr. Hans-Henning Steinbiß
Max-Planck-Institut für Züchtungsforschung (MPIZ)
Carl-von-Linné-Weg 10, 50829 Köln
Tel: 0221 5062 210/211
Fax: 0221 5062 213
Clash marker genes
Research projects
New methods for gene transfer 2001-2004
- Targeted insertion of genes, University of Karlsruhe
- Development of new marker genes, SunGene
- Cutting out undesired genes with the help of jumping genes, Planta
- Cutting out undesired genes: Cre/lox-System, BBA Braunschweig
- Cutting out undesired genes with the help of a novel recombination system, Bavarian State Research Center for Agriculture, Freising
- Negative selection marker, University of Rostock
- Plant microinjection, University of Giessen
- Appropriate plant cells for microinjection, Bioplant
- Genes for microinjection, Bioplant
- Microinjection, FI Schmallenberg
- Targeted modification of genes in plants, BBA Braunschweig
- Biosafety system for the production of proteins in plants with modified viruses, BBA Braunschweig
- Optimisation of binary vectors, BfZ Siebeldingen
- Marker gene-free plants through out-crossing, MPIZ Köln
- Transformation in plastids, SunGene
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