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Journal of Bacteriology, September 1998, p. 4583-4590, Vol. 180, No. 17
Departamento de Microbiología del
Suelo y Sistemas Simbióticos, Estación Experimental del
Zaidín, CSIC, E-18008 Granada, Spain
Received 6 February 1998/Accepted 12 June 1998
A simple approach was used to identify Rhizobium
meliloti DNA regions with the ability to convert a
nontransmissible vector into a mobilizable plasmid, i.e., to
contain origins of conjugative transfer (oriT,
mob). RecA-defective R. meliloti merodiploid
populations, where each individual contained a hybrid cosmid from an
R. meliloti GR4 gene library, were used as donors en masse
in conjugation with another R. meliloti recipient strain,
selecting transconjugants for vector-encoded antibiotic resistance.
Restriction analysis of cosmids isolated from individual
transconjugants resulted in the identification of 11 nonoverlapping DNA
regions containing potential oriTs. Individual hybrid
cosmids were confirmed to be mobilized from the original
recA donors at frequencies ranging from 10
0021-9193/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
Cloning and Identification of Conjugative Transfer
Origins in the Rhizobium meliloti Genome
2
to 10
5 per recipient cell. DNA hybridization experiments
showed that seven mob DNA regions correspond to plasmid
replicons: four on symbiotic megaplasmid 1 (pSym1), one on pSym2, and
another two on each of the two cryptic plasmids harbored by R. meliloti GR4. Another three mob clones could not be
located to any plasmid and were therefore preliminarily assigned to the
chromosome. With this strategy, we were able to characterize the
oriT of the conjugative plasmid pRmeGR4a, which confirmed
the reliability of the approach to select for oriTs.
Moreover, transfer of the 11 mob cosmids from R. meliloti into Escherichia coli occurred at
frequencies as high as 10
1, demonstrating the R. meliloti gene transfer capacity is not limited to the family
Rhizobiaceae. Our results show that the R. meliloti genome contains multiple oriTs that allow
efficient DNA mobilization to rhizobia as well as to phylogenetically
distant gram-negative bacteria.
*
Corresponding author. Mailing address: Departamento de
Microbiología, Estación Experimental del
Zaidín-CSIC, Prof. Albareda 1, E-18008 Granada, Spain. Phone:
34-958-121011. Fax: 34-958-129600. E-mail:
Juan.Sanjuan{at}eez.csic.es.
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