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An RP4-prime containing a 285 kb fragment of rhizobium meliloti pSym megaplasmid: Structural characterization and utilization for genetic studies of symbiotic functions controlled by pSym
Authors:J S Julliot  Ilona Dusha  Marie Hélène Renalier  Betty Terzaghi  Anne Marie Garnerone and P Boistard
Institution:(1) Laboratoire de Biologie Moléculaire des Relations Plantes Microorganismes CNRS INRA, Groupement Scientifique Microbiologie Toulouse, BP 12, F-31320 Castanet Tolosan, France;(2) Present address: Institute of Genetics Biological Research Center, Hungarian Academy of Sciences, Szeged, Hungary;(3) Present address: Plant Physiology Division, DSIR, Private Bag, Palmerston North, New Zealand
Abstract:Summary We integrated the RP4 plasmid into a selected region of the pSym megaplasmid of Rhizobium meliloti 2011 by homologous recombination between pSym and a cloned fragment of pSym present in the RP4. This cointegrate was used to mobilize into Escherichia coli a Tn5 transposon located on pSym in the vicinity of the site of integration of the RP4. By this technique we obtained a series of RP4-primes that contained large fragments of the pSym megaplasmid and that were most probably generated by IS8 promoted deletions in the RP4-pSym cointegrate. One of them, pGMI42, which carries nitrogenase genes nifD and H as well as nodulation genes, was used for mutagenesis of the corresponding region of pSym after insertion of the Mu prophage into the tet gene. When various (pGMI-42:: Mu)::Tn7 were introduced into R. meliloti 2011 by conjugation, homologous recombination allowed insertion of Tn7 into pSym whereas the pGMI42::Mu was lost due to the suicide effect of Mu. In this way we obtained several symbiotic mutants deficient in either nodulation (Nod-) or nitrogen fixation (Fix-) in association with the host plant Medicago sativa.This paper is affectionately dedicated to the memory of Jean-Simon Julliot who initiated and inspired this work and who was killed by an avalanche on February 21, 1982
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