1986
DOI: 10.1128/jb.167.1.66-72.1986
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Second symbiotic megaplasmid in Rhizobium meliloti carrying exopolysaccharide and thiamine synthesis genes

Abstract: Using physical and genetic data, we have demonstrated that Rhizobium meliloti SU47 has a symbiotic megaplasmid, pRmeSU47b, in addition to the previously described nod-nif megaplasmid pRmeSU47a. This plasm'id includes four loci involved in exopolysaccharide (exo) synthesis as well as two loci involved in thiamine 1'iosynthesis. Mutations at the exo loci have previously been shown to result in the formation of nodules which lack infection threads (Inf)' and fail to fix nitrogen (Fix-). Thus, both megaplasmids co… Show more

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Cited by 574 publications
(369 citation statements)
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“…D-Glucose or L-arabinose (0.2%) was added to repress or induce, respectively, the expression of genes under the control of the P BAD promoter (Guzman et al, 1995). Plasmids were mobilized from E. coli to C. crescentus by bacterial conjugation with the help of pRK600 (Finan et al, 1986).…”
Section: Bacterial Strains Plasmids and Growth Conditionsmentioning
confidence: 99%
“…D-Glucose or L-arabinose (0.2%) was added to repress or induce, respectively, the expression of genes under the control of the P BAD promoter (Guzman et al, 1995). Plasmids were mobilized from E. coli to C. crescentus by bacterial conjugation with the help of pRK600 (Finan et al, 1986).…”
Section: Bacterial Strains Plasmids and Growth Conditionsmentioning
confidence: 99%
“…The disrupted sdeB and sdeR fragments were transferred into the pKNG101 replacement vector and cloned into E. coli CC118 in a similar fashion as for hasF. Conjugation between the E. coli strain harbouring each of the disrupted S. marcescens sdeB, hasF and sdeR genes and the wild-type S. marcescens strain was carried out using E. coli helper strain MT616 (Finan et al, 1986) to create SDEAB1, HASF100 and SDER1, respectively. Conjugation was also carried out between the E. coli strain harbouring each of the disrupted S. marcescens sdeB and hasF genes and the S. marcescens clinical isolate strain (T-861), using E. coli helper strain MT616 (Finan et al, 1986) for comparison purposes.…”
Section: Methodsmentioning
confidence: 99%
“…Conjugation between the E. coli strain harbouring each of the disrupted S. marcescens sdeB, hasF and sdeR genes and the wild-type S. marcescens strain was carried out using E. coli helper strain MT616 (Finan et al, 1986) to create SDEAB1, HASF100 and SDER1, respectively. Conjugation was also carried out between the E. coli strain harbouring each of the disrupted S. marcescens sdeB and hasF genes and the S. marcescens clinical isolate strain (T-861), using E. coli helper strain MT616 (Finan et al, 1986) for comparison purposes. For the double sdeB/hasF-deficient mutant (SDEAB3/HASF300), conjugation was carried out between the S. marcescens sdeB (SDEAB1)-and hasF (HASF100)-deficient strains, using E. coli MT616 as a helper.…”
Section: Methodsmentioning
confidence: 99%
“…Interestingly, the size of the g. iaponicum genes for an essential biochemical pathway, the thiamine biosynthesis pathway, have been localized to a megaplasmid in R. meliloti (Finan et al, 1986). I believe that R. meliloti 1021 probably has three essential replicons in its genome, which should be called chromosomes, by definition, and that there is a large degree of genetic exchange between these replicons (Burkardt et al, 1987).…”
Section: General Summarymentioning
confidence: 99%
“…meliloti (Finan et al, 1986). Based on electron microscope (EM) contour measurements of large samples of megaplasmids, Burkardt et al (1987) Although E-meliloti is the most thoroughly studied of the…”
mentioning
confidence: 99%