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Plant Physiol, May 2003, Vol. 132, pp. 174-184 Chimeric RNA/DNA Oligonucleotide-Based Site-Specific Modification of the Tobacco Acetolactate Syntase GeneMax-Planck-Institute of Molecular Plant Physiology, Am Mühlenberg 1, 14476 Golm, Germany
Single amino acid substitutions at either of two crucial
positions in acetolactate synthase (ALS) result in a
chlorsulfuron-insensitive form of this enzyme and, as a consequence, a
herbicide-resistant phenotype. Here, we describe the successful in vivo
targeting of endogenous tobacco (Nicotiana tabacum) ALS
genes using chimeric RNA/DNA and all-DNA oligonucleotides at two
different locations. Similar number of conversion events with two
different chimeras indicates the absence of restricting influence of
genomic target sequence on the gene repair in tobacco.
Chlorsulfuron-resistant plants were regenerated from calli after
mesophyll protoplast electroporation or leaf tissue particle
bombardment with these specifically constructed chimeras. Sequence
analysis and enzyme assays proved the resulting alterations to ALS at
both DNA and protein levels. Furthermore, foliar application of
chlorsulfuron confirmed the development of resistant phenotypes. Lines
with proline-196-alanine, threonine, glutamine, or serine substitutions or with tryptophan-573-leucine substitutions were highly resistant at
both cellular and whole plant levels, whereas lines with
proline-196-leucine substitutions were less resistant. The stability of
these modifications was demonstrated by the continuous growth of calli
on chlorsulfuron-containing medium and by the transmission of herbicide
resistance to progeny in a Mendelian manner. Ability of haploid state
to promote chimera-mediated conversions is discussed.
* Corresponding author; e-mail kochevenko{at}mpimp-golm.mpg.de; fax 49-331-567-8408. © 2003 American Society of Plant Biologists This article has been cited by other articles:
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