Symbiotic Plasmid Rearrangement in Rhizobium leguminosarum bv. viciae VF39SM

doi:10.1128/JB.183.6.2141-2144.2001

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Journal of Bacteriology, March 2001, p. 2141-2144, Vol. 183, No. 6
0021-9193/01/$04.00+0 DOI: 10.1128/JB.183.6.2141-2144.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Symbiotic Plasmid Rearrangement in Rhizobium leguminosarum bv. viciae VF39SM

Xue-Xian Zhang, Bob Kosier, and Ursula B. Priefer^*

Ökologie des Bodens, Institut für Botanik, RWTH Aachen, 52060 Aachen, Germany

Received 17 August 2000/Accepted 14 December 2000

	ABSTRACT

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A rearrangement between the symbiotic plasmid (pRleVF39d) and a nonsymbiotic plasmid (pRleVF39b) in Rhizobium leguminosarumbv. viciae VF39 was observed. The rearranged derivative showedthe same plasmid profile as its parent strain, but hybridizationto nod, fix, and nif genes indicated that most of the symbioticgenes were now present on a plasmid corresponding in size to pRleVF39binstead of pRleVF39d. On the other hand, some DNA fragments originatingfrom pRleVF39b now hybridized to the plasmid band at the positionof pRleVF39d. These results suggest that a reciprocal but unequalDNA exchange between the two plasmids hadoccurred.

	TEXT

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Rhizobium leguminosarum bv. viciae is a native soil bacterium that can enter nitrogen-fixing symbioses (root nodules) withseveral legumes such as Pisum, Vicia, and Lens spp. It generallycontains 1 to 10 plasmids which vary in size from 30 kb to morethan 800 kb (11, 12, 14). Most of the genes required fornodule formation (nod) and nitrogen fixation (nif and fix) arecarried on a plasmid that is traditionally called the symbioticplasmid or pSym (6, 11).

Plasmids are important genetic components for the divergence and adaptation of microbial populations because they contributeto genomic plasticity. Although plasmid profiles in rhizobia canbe considered as a comparatively stable character, strains canlose some of their traits due to loss or partial deletion of aplasmid (3, 27). Recombination and rearrangement events betweenplasmids is also frequently observed. For example, for R. leguminosarumbv. viciae it was found that a transmissible plasmid could pickup symbiotic determinants from the nontransmissible pSym (1),and pSym rearrangements have been described and studied in detailin R. etli and R. tropici (2, 4, 21, 22). One of theserearrangements is a deletion of the symbiotic gene region, accompaniedby a concomitant amplification of other sequences, so that theoverall size of the plasmid is not significantly changed (21).

In this study, we present direct evidence of a DNA rearrangement between two indigenous plasmids of R. leguminosarum bv. viciaeVF39SM, a model strain that is routinely used in our laboratory(Table 1). It contains six plasmids, ranging in size from 130kb to approximately 600 kb (9). They were designated as pRleVF39ato pRleVF39f in order of increasing molecular size. The symbioticplasmid pRleVF39d carries the nod, nif, and most of the fix genes(9, 10). Some fix genes, such as fixKL and a second copyof the fixNOQP operon, reside on plasmid pRleVF39c, which alsocarries genes involved in lipopolysaccharide synthesis (10,15, 24). Little is known about pRleVF39b except that it carriesa restriction-modification system (20) and that it is self-transmissible(9).

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TABLE 1. Bacterial strains and plasmids used in this study

Hybridization analyses reveal a pSym rearrangement. The rearrangement described here was found when single colonies of the original VF39SM stock culture, stored in 20% glycerolat $-$ 20°C since 1993, were checked by plasmid profiling using amodified Eckhardt procedure (8, 16) and subsequent Southernhybridization analysis with nodABC genes as a probe. The digoxigenin-labeledprobe was prepared via PCR by using primers pnodA (5'-AGT GCGATG GAA AAT ATG CTG-3') and pnodC (5'-GGA AGC GCA AGC AAA GTATC-3'), which correspond to positions 4521 to 4541 and positions2376 to 2395, respectively, in the pRl1JI nodABC sequence (accessionnumber X99520). Although all isolates showed the plasmid patterncharacteristic for VF39SM (Fig. 1A), 1 out of 100 colonies wasidentified in which hybridization to nodABC occurred to a plasmidcorresponding in size to pRleVF39b (240 kb), whereas in all theothers the hybridization was as expected to pRleVF39d (pSym, 330kb) (Fig. 1B). This result suggested the event of a DNA rearrangementin this isolate. Therefore, it was renamed VF39SM' (Table 1),and its plasmids were accordingly renamed pRleVF39a' to pRleVF39f'.

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FIG. 1. Profiles and hybridization results of the plasmids in R. leguminosarum bv. viciae VF39SM (lane 1) and its rearranged derivative VF39SM' (lane 2). (A) Eckhardt gel showing the banding pattern of the six plasmids (negative image); their designation (for the parental VF39SM strain) and the estimated sizes of the plasmid bands are given on the left. (B to H) Hybridization results of the plasmid gels with nodABC (B), nodO (C), fixLKNO (D), fixBCX-nifA (E), pXTZ11 (F), pXTZ12 (G), and repC (H).

To estimate the extent of this rearrangement, the localization of other symbiotic genes was analyzed. Southern hybridizationwith a nodO probe, amplified and labeled using primers pnodO1(5'-CGT AAG CGA GGT AAG ATC CG-3') and pnodO2 (5'-AGA ACG ACTGGA TTG ATG CC-3'), which were designed on the basis of the pRL1JIsequence (accession number X17285), indicated that in VF39SM'this gene was now also carried on the 240-kb plasmid instead ofpRleVF39d (Fig. 1C). When the fixLKNO gene region was used asa probe, a strong signal with plasmid pRleVF39c, which carriesone copy of the fixNOQP operon upstream of the fixKL region (15,24), was observed for both strains; the second copy of fixNOQP,however, which normally is carried on pRleVF39d in VF39SM (24)was detected at the position of pRleVF39b' in the rearranged strain(Fig. 1D; the hybridization signals of this copy are weak becauseit does not contain the fixLK genes). Likewise, hybridizationto the fixBCX-nifA genes had changed from pRleVF39d to pRleVF39b'(Fig. 1E). These results suggest that in the rearranged strainVF39SM' almost the entire symbiotic region originally presenton plasmid pRleVF39d is now carried on a plasmid banding at positionpRleVF39b'.

Plant tests with Vicia hirsuta confirmed that the two strains had similar symbiotic properties with respect to nodule formation,acetylene reduction activity, and plant shoot dry weights (datanotshown).

The rearrangement occurred by reciprocal but unequal exchange of DNA. To test whether there was also a shift in the hybridization pattern of sequences originally carried by plasmid pRleVF39b,DNA of the parental pRleVF39b plasmid was isolated from the Eckhardtgel, digested completely with XhoI and HindIII, and cloned intovector pXT (7). Four clones (pXTZ11 to pXTZ14 [Table 1]),which contained 600-bp to 2.8-kb inserts, were randomly chosenand used to probe the plasmids of VF39SM and VF39SM'. The 2.5-kbDNA fragment cloned in pXTZ11 hybridized to the 240-kb plasmidin both strains (Fig. 1F); pXTZ12, pXTZ13, and pXTZ14 hybridizedto plasmid pRleVF39b in the parental strain but to the pRleVF39d'band in the rearranged derivative (exemplified for pXTZ12 in Fig.1G; in both strains, pXTZ12 also gave a weak hybridization topRleVF39a). These data suggest that the two plasmids had exchangedgeneticinformation.

Since the DNA arrangement did not visibly change the overall plasmid profile of the strain, it could have occurred in twopossible ways. The first is that the two plasmids have exchangeda DNA region of exactly the same size, which would mean that plasmidpRleVF39d' is a rearranged version of the original pSym (now withoutthe sym region and containing part of pRleVF39b instead) and thatthe plasmid pRleVF39b' represents plasmid pRleVF39b, which hasacquired the sym gene region from plasmid pRleVF39d in exchangefor its own DNA of the same size. The alternative possibilityis that the DNA region obtained by plasmid pRleVF39b exceeds theregion transferred to plasmid pRleVF39d by 90 kb, thus shiftingthe size of plasmid pRleVF39b from 240 to 330 kb (i.e., to thegel position of pRleVF39d) and decreasing the size of pRleVF39daccordingly. This would mean that in VF39SM' the plasmid bandwith a size of 240 kb (pRleVF39b') is actually a rearranged versionof pSym (pRleVF39d) still containing the symregion.

To determine which possibility had occurred, the replication regions of the two plasmids were analyzed. By using a pair ofconserved PCR primers, RC1 and RC3, developed to amplify repCgenes of R. leguminosarum (19, 26), a product with the expectedsize of 750 bp was amplified from total DNA of VF39SM, and itwas used as a probe to hybridize the plasmid gels. As shown inFig. 1H, the repC probe was found to hybridize to pRleVF39d inVF39SM and to pRleVF39b' in VF39SM'. This means that the symbioticgenes are still contained on the original replicon, suggestingthat the rearrangement had occurred by the second way describedabove.

Since several copies of a putative insertion sequence (ISRle39) were found to be present on plasmid pRleVF39b (20), we testedwhether these elements were involved in the DNA rearrangement.ISRle39 was amplified from total VF39SM DNA and used as a hybridizationprobe. In VF39SM, a strong signal was found to plasmid pRleVF39b(and also to plasmid pRleVF39a), whereas in VF39SM' the signalhad shifted to the position of pRleVF39d' (data not shown). Providedthat the rearrangement had occurred by the second mechanism proposed(i.e., that the plasmid band designated pRleVF39d' correspondsto the rearranged pRleVF39b plasmid), this would mean that theseIS elements have not been part of the DNAexchange.

It was also checked whether further rearrangements could occur. For this purpose, 50 single colonies of strain VF39SM' werestudied by plasmid profile and nodABC Southern hybridization analyses.A deletion in plasmid pRleVF39b' of about 45 kb was detected inone colony (VF39SM"). No hybridization signal to nodABC was foundin this deletion derivative and it failed to nodulate V. hirsuta,indicating that the deleted DNA region included the nodulationgenes. All other colonies had normal plasmid profiles, and theirnod genes were still located on pRleVF39b'.

Delineation of one rearrangement site. By using cosmid 220 (kindly provided by M. F. Hynes), which contains a 30-kb insert from pRleVF39b, and appropriate subclonesthereof, a 2.2-kb BamHI/HindIII fragment was identified that hybridizedonly to pRleVF39b in the original strain but to both pRleVF39b'and pRleVF39d' in VF39SM' (data not shown), suggesting that thisregion was involved in the generation of the rearrangement. DNAsequence analysis (accession number AJ292764) revealed an openreading frame (ORF1) with 73% homology, at both the DNA and aminoacid levels, to Y4JO, a hypothetical 36.1-kDa protein encodedby pNGR234a from Sinorhizobium sp. strain NGR234 (accession numberAE000080, positions 3600 to 4646). Y4JO may be a fragment ofa larger protein of as-yet-unknown function (5). It is notablethat the C-terminal part of ORF1 (positions 324 to 359) shows69% homology at protein level with the C-terminal end of a putativetransposase of Vibrio cholerae (accession number AB012957),suggesting that the ORF1 gene product may have some function inthe observed DNA rearrangement, which will be studied in the future.Considering that the other sequences upstream and downstream ofORF1 show no homology with the neighboring sequences of Y4JO,it seems that this DNA region has undergone recombination severaltimes.

Although at present, the molecular mechanisms leading to the rearrangement described here are not understood, the data presentedimply that it is caused by a reciprocal but unequal exchange ofDNA, resulting in a decrease in the size of pSym and a simultaneousincrease in the size of pRleVF39b. Symbiotic plasmid rearrangementhave been previously described in field isolates of Sinorhizobiummeliloti (18) and R. leguminosarum (23, 25). Mazurier andLaguerre (13) recently reported an unusual location of symbioticgenes in some R. leguminosarum bv. viciae field isolates, whichcould be the result of genome rearrangements between the pSymand another replicon. Our own work on the pSym diversity amongR. leguminosarum field isolates indicated that identical sym genegenotypes can be carried by plasmids of different sizes, rangingfrom 190 to 630 kb (unpublished data). These findings suggestthat plasmid DNA rearrangements similar to that described heremay also occur in the naturalenvironment.

	ACKNOWLEDGMENTS

We thank M. F. Hynes (University of Calgary, Calgary, Ontario, Canada) for fruitful discussions and for providing cosmid clone220. We also thank A. Seibold for helpful technical advice andassistance and B. Boesten for constructivecriticism.

X.-X. Zhang was supported by an Alexander-von-Humboldtfellowship.

	FOOTNOTES

^* Corresponding author. Mailing address: Ökologie des Bodens, Institut für Botanik, RWTH, Aachen, Worringer Weg 1, 52060 Aachen,Germany. Phone: 49-241-80-6644. Fax: 49-241-8888-637. E-mail:priefer{at}bio1.rwth-aachen.de.

Present address: Center for Ecology and Hydrology, Oxford OX1 3SR, UnitedKingdom.

REFERENCES

Top
Abstract
Text
References

1. Brewin, N. J., E. A. Wood, A. W. B. Johnston, N. J. Dibb, and G. Hombrecher. 1982. Recombinant nodulation plasmids in Rhizobium leguminosarum. J. Gen. Microbiol. 128:1817-1827.

2. Brom, S., A. García de los Santos, M. L. Girard, G. Dávila, R. Palacios, and D. Romero. 1991. High-frequency rearrangements in Rhizobium leguminosarum bv. phaseoli plasmids. J. Bacteriol. 173:1344-1346[Abstract/Free Full Text].

3. Djordjevic, M. A., W. Zurkowski, and B. G. Rolfe. 1982. Plasmids and stability of symbiotic properties of Rhizobium trifolii. J. Bacteriol. 151:560-568[Abstract/Free Full Text].

4. Flores, M., V. González, M. A. Pardo, A. Leija, E. Martínez, D. Romero, D. Pinero, G. Dávila, and R. Palacios. 1988. Genomic instability in Rhizobium phaseoli. J. Bacteriol. 170:1191-1196[Abstract/Free Full Text].

5. Freiberg, C., R. Fellay, A. Bairoch, W. J. Broughton, A. Rosenthal, and X. Perret. 1997. Molecular basis of symbiosis between Rhizobium and legumes. Nature 387:394-401[CrossRef][Medline].

6. García de los Santos, A., S. Brom, and D. Romero. 1996. Rhizobium plasmids in bacteria-legume interactions. World J. Microbiol. Biotechnol. 12:119-125.

7. Harrison, J., P. L. Molloy, and S. J. Clark. 1994. Direct cloning of polymerase chain reaction products in an XcmI T-vector. Anal. Biochem. 216:235-236[CrossRef][Medline].

8. Hynes, M. F., R. Simon, and A. Pühler. 1985. The development of plasmid-free strains of Agrobacterium tumefaciens by using incompatibility with a Rhizobium meliloti plasmid to eliminate pAEC58. Plasmid 13:99-105[CrossRef][Medline].

9. Hynes, M. F., K. Brucksch, and U. B. Priefer. 1988. Melanin production encoded by a cryptic plasmid in a Rhizobium leguminosarum strain. Arch. Microbiol. 150:326-332[CrossRef].

10. Hynes, M. F., and N. F. McGregor. 1990. Two plasmids other than the nodulation plasmid are necessary for formation of nitrogen-fixing nodules by Rhizobium leguminosarum. Mol. Microbiol. 4:567-574[Medline].

11. Martínez-Romero, E., and R. Palacios. 1990. The Rhizobium genome. Crit. Rev. Plant Sci. 9:59-93.

12. Martínez-Romero, E., and J. Caballero-Mellado. 1996. Rhizobium phylogenies and bacterial genetic diversity. Crit. Rev. Plant Sci. 15:113-140.

13. Mazurier, S. I., and G. Laguerre. 1997. Unusual location of nod and nif genes in Rhizobium leguminosarum bv. viciae. Can. J. Microbiol. 43:399-402.

14. Mercado-Blanco, J., and N. Toro. 1996. Plasmids in rhizobia: the role of nonsymbiotic plasmids. Mol. Plant-Microbe Interact. 9:535-545.

15. Patschkowski, T., A. Schlüter, and U. B. Priefer. 1996. Rhizobium leguminosarum bv. viciae contains a second fnr/fixK-like gene and an unusual fixL homologue. Mol. Microbiol. 21:267-280[CrossRef][Medline].

16. Priefer, U. B. 1984. Isolation of plasmid DNA, p. 14-24. In A. Pühler, and K. N. Timmis (ed.), Advanced molecular genetics. Springer-Verlag, Berlin, Germany.

17. Priefer, U. B. 1989. Genes involved in lipopolysaccharide production and symbiosis are clustered on the chromosome of Rhizobium leguminosarum bv. viciae VF39. J. Bacteriol. 171:6161-6168[Abstract/Free Full Text].

18. Rastogi, V. K., E. S. P. Bromfield, S. T. Whitwill, and L. R. Barran. 1992. A cryptic plasmid of indigenous Rhizobium meliloti possesses reiterated nodC and nifE genes and undergoes DNA arrangement. Can. J. Microbiol. 38:563-568.

19. Rigottier-Gois, L., S. L. Turner, J. P. W. Young, and N. Amarger. 1998. Distribution of repC plasmid-replication sequences among plasmids and isolates of Rhizobium leguminosarum bv. viciae from field populations. Microbiology 144:771-780[Abstract/Free Full Text].

20. Rochepeau, P., L. B. Selinger, and M. F. Hynes. 1997. Transposon-like structure of a new plasmid-encoded restriction-modification system in Rhizobium leguminosarum VF39SM. Mol. Gen. Genet. 256:387-396[CrossRef][Medline].

21. Romero, D., S. Brom, J. Martínez-Salazar, M. L. Girard, R. Palacios, and G. Dávila. 1991. Amplification and deletion of a nod-nif region in the symbiotic plasmid of Rhizobium phaseoli. J. Bacteriol. 173:2435-2441[Abstract/Free Full Text].

22. Romero, D., J. Martínez-Salazar, L. Girard, S. Brom, G. Dávila, R. Palacios, M. Flores, and C. Rodriguez. 1995. Discrete amplifiable regions (amplicons) in the symbiotic plasmid of Rhizobium etli CFN42. J. Bacteriol. 177:973-980[Abstract/Free Full Text].

23. Schofield, P. R., A. H. Gibson, W. F. Dudman, and J. M. Watson. 1987. Evidence for genetic exchange and recombination of Rhizobium symbiotic plasmids in a soil population. Appl. Environ. Microbiol. 53:2942-2947[Abstract/Free Full Text].

24. Schlüter, A., T. Patschkowski, J. Quandt, L. B. Selinger, S. Weidner, M. Krämer, L. M. Zhou, M. F. Hynes, and U. B. Priefer. 1997. Functional and regulatory analysis of the two copies of the fixNOQP operon of Rhizobium leguminosarum strain VF39. MPMI 10:605-616.

25. Selbitscka, W., and W. Lotz. 1991. Instability of cryptic plasmids affects the symbiotic efficiency of Rhizobium leguminosarum bv. viciae strains. Mol. Plant-Microbe Interact. 4:608-618.

26. Turner, S. L., L. Rigottier-Gois, R. S. Power, N. Amarger, and J. P. W. Young. 1996. Diversity of recC plasmid-replication sequences in Rhizobium leguminosarum. Microbiology 142:1705-1713[Abstract/Free Full Text].

27. Weaver, R. W., G. R. Wei, and D. L. Berryhill. 1990. Stability of plasmids in R. phaseoli during culture. Soil Biol. Biochem. 22:465-469[CrossRef].

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1.	Brewin, N. J., E. A. Wood, A. W. B. Johnston, N. J. Dibb, and G. Hombrecher. 1982. Recombinant nodulation plasmids in Rhizobium leguminosarum. J. Gen. Microbiol. 128:1817-1827.
2.	Brom, S., A. García de los Santos, M. L. Girard, G. Dávila, R. Palacios, and D. Romero. 1991. High-frequency rearrangements in Rhizobium leguminosarum bv. phaseoli plasmids. J. Bacteriol. 173:1344-1346[Abstract/Free Full Text].
3.	Djordjevic, M. A., W. Zurkowski, and B. G. Rolfe. 1982. Plasmids and stability of symbiotic properties of Rhizobium trifolii. J. Bacteriol. 151:560-568[Abstract/Free Full Text].
4.	Flores, M., V. González, M. A. Pardo, A. Leija, E. Martínez, D. Romero, D. Pinero, G. Dávila, and R. Palacios. 1988. Genomic instability in Rhizobium phaseoli. J. Bacteriol. 170:1191-1196[Abstract/Free Full Text].
5.	Freiberg, C., R. Fellay, A. Bairoch, W. J. Broughton, A. Rosenthal, and X. Perret. 1997. Molecular basis of symbiosis between Rhizobium and legumes. Nature 387:394-401[CrossRef][Medline].
6.	García de los Santos, A., S. Brom, and D. Romero. 1996. Rhizobium plasmids in bacteria-legume interactions. World J. Microbiol. Biotechnol. 12:119-125.
7.	Harrison, J., P. L. Molloy, and S. J. Clark. 1994. Direct cloning of polymerase chain reaction products in an XcmI T-vector. Anal. Biochem. 216:235-236[CrossRef][Medline].
8.	Hynes, M. F., R. Simon, and A. Pühler. 1985. The development of plasmid-free strains of Agrobacterium tumefaciens by using incompatibility with a Rhizobium meliloti plasmid to eliminate pAEC58. Plasmid 13:99-105[CrossRef][Medline].
9.	Hynes, M. F., K. Brucksch, and U. B. Priefer. 1988. Melanin production encoded by a cryptic plasmid in a Rhizobium leguminosarum strain. Arch. Microbiol. 150:326-332[CrossRef].
10.	Hynes, M. F., and N. F. McGregor. 1990. Two plasmids other than the nodulation plasmid are necessary for formation of nitrogen-fixing nodules by Rhizobium leguminosarum. Mol. Microbiol. 4:567-574[Medline].
11.	Martínez-Romero, E., and R. Palacios. 1990. The Rhizobium genome. Crit. Rev. Plant Sci. 9:59-93.
12.	Martínez-Romero, E., and J. Caballero-Mellado. 1996. Rhizobium phylogenies and bacterial genetic diversity. Crit. Rev. Plant Sci. 15:113-140.
13.	Mazurier, S. I., and G. Laguerre. 1997. Unusual location of nod and nif genes in Rhizobium leguminosarum bv. viciae. Can. J. Microbiol. 43:399-402.
14.	Mercado-Blanco, J., and N. Toro. 1996. Plasmids in rhizobia: the role of nonsymbiotic plasmids. Mol. Plant-Microbe Interact. 9:535-545.
15.	Patschkowski, T., A. Schlüter, and U. B. Priefer. 1996. Rhizobium leguminosarum bv. viciae contains a second fnr/fixK-like gene and an unusual fixL homologue. Mol. Microbiol. 21:267-280[CrossRef][Medline].
16.	Priefer, U. B. 1984. Isolation of plasmid DNA, p. 14-24. In A. Pühler, and K. N. Timmis (ed.), Advanced molecular genetics. Springer-Verlag, Berlin, Germany.
17.	Priefer, U. B. 1989. Genes involved in lipopolysaccharide production and symbiosis are clustered on the chromosome of Rhizobium leguminosarum bv. viciae VF39. J. Bacteriol. 171:6161-6168[Abstract/Free Full Text].
18.	Rastogi, V. K., E. S. P. Bromfield, S. T. Whitwill, and L. R. Barran. 1992. A cryptic plasmid of indigenous Rhizobium meliloti possesses reiterated nodC and nifE genes and undergoes DNA arrangement. Can. J. Microbiol. 38:563-568.
19.	Rigottier-Gois, L., S. L. Turner, J. P. W. Young, and N. Amarger. 1998. Distribution of repC plasmid-replication sequences among plasmids and isolates of Rhizobium leguminosarum bv. viciae from field populations. Microbiology 144:771-780[Abstract/Free Full Text].
20.	Rochepeau, P., L. B. Selinger, and M. F. Hynes. 1997. Transposon-like structure of a new plasmid-encoded restriction-modification system in Rhizobium leguminosarum VF39SM. Mol. Gen. Genet. 256:387-396[CrossRef][Medline].
21.	Romero, D., S. Brom, J. Martínez-Salazar, M. L. Girard, R. Palacios, and G. Dávila. 1991. Amplification and deletion of a nod-nif region in the symbiotic plasmid of Rhizobium phaseoli. J. Bacteriol. 173:2435-2441[Abstract/Free Full Text].
22.	Romero, D., J. Martínez-Salazar, L. Girard, S. Brom, G. Dávila, R. Palacios, M. Flores, and C. Rodriguez. 1995. Discrete amplifiable regions (amplicons) in the symbiotic plasmid of Rhizobium etli CFN42. J. Bacteriol. 177:973-980[Abstract/Free Full Text].
23.	Schofield, P. R., A. H. Gibson, W. F. Dudman, and J. M. Watson. 1987. Evidence for genetic exchange and recombination of Rhizobium symbiotic plasmids in a soil population. Appl. Environ. Microbiol. 53:2942-2947[Abstract/Free Full Text].
24.	Schlüter, A., T. Patschkowski, J. Quandt, L. B. Selinger, S. Weidner, M. Krämer, L. M. Zhou, M. F. Hynes, and U. B. Priefer. 1997. Functional and regulatory analysis of the two copies of the fixNOQP operon of Rhizobium leguminosarum strain VF39. MPMI 10:605-616.
25.	Selbitscka, W., and W. Lotz. 1991. Instability of cryptic plasmids affects the symbiotic efficiency of Rhizobium leguminosarum bv. viciae strains. Mol. Plant-Microbe Interact. 4:608-618.
26.	Turner, S. L., L. Rigottier-Gois, R. S. Power, N. Amarger, and J. P. W. Young. 1996. Diversity of recC plasmid-replication sequences in Rhizobium leguminosarum. Microbiology 142:1705-1713[Abstract/Free Full Text].
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