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Expression in transgenic tobacco of the bacterial neomycin phosphotransferase gene modified by intron insertions of various sizes
Authors:Jerzy Paszkowski  Alex Peterhans  Roland Bilang  Witold Filipowicz
Affiliation:(1) Institute of Plant Sciences, Swiss Federal Institute of Technology, ETH-Zentrum, CH-8092 Zürich, Switzerland;(2) Friedrich Miescher Institute, P.O. Box 2543, CH-4002 Basel, Switzerland
Abstract:A plant selectable marker gene consisting of cauliflower mosaic virus expression signals and the proteincoding sequence of bacterial neomycin phosphotransferase was modified by insertion of an intron sequence from a storage protein gene, phaseolin. Correct and efficient splicing of the resulting mosaic RNA was observed in transgenic tobacco plants. The insertion of various linkers or gradual increase of intron size by addition in both orientations of internal intron sequences from another plant gene (parsley, 4-coumarate ligase) had little or no effect on the precision of slicing. The gene activity measured by selectability assay in the protoplast transformation showed that only introns enlarged to 1161 bases and longer caused decreased selectability. The suitability of such mosaic marker genes for studies of RNA splicing, DNA recombination and early events after infection of plants with Agrobacterium is discussed.
Keywords:transgenic tobacco plants  RNA splicing  protoplast transformation
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