Literature DB >> 7545154

Lateral transfer of rfb genes: a mobilizable ColE1-type plasmid carries the rfbO:54 (O:54 antigen biosynthesis) gene cluster from Salmonella enterica serovar Borreze.

W J Keenleyside1, C Whitfield.   

Abstract

Plasmid pWQ799 is a 6.9-kb plasmid isolated from Salmonella enterica serovar Borreze. Our previous studies have shown that the plasmid contains a functional biosynthetic gene cluster for the expression of the O:54 lipopolysaccharide O-antigen of this serovar. The minimal replicon functions of pWQ799 have been defined, and a comparison with nucleotide and protein databases revealed this replicon to be virtually identical to ColE1. This is the first report of involvement of ColE1-related plasmids in O-antigen expression. The replicon of pWQ799 is predicted to encode two RNA molecules, typical of other ColE1-type plasmids. RNAII, the putative replication primer from pWQ799, shares regions of homology with RNAII from ColE1. RNA1 is an antisense regulator of DNA replication in ColE1-related plasmids. The coding region for RNAI from pWQ799 shares no homology with any other known RNAI sequence but is predicted to adopt a secondary structure characteristic of RNAI molecules. pWQ799 may therefore represent a new incompatibility group within this family. pWQ799 also possesses cer, rom, and mob determinants, and these differ minimally from those of ColE1. The plasmid is mobilizable in the presence of either the broad-host-range helper plasmid pRK2013 or the IncI1 plasmid R64drd86. Mobilization and transfer of pWQ799 to other organisms provides the first defined mechanism for lateral transfer of O-antigen biosynthesis genes in S. enterica and explains both the distribution of related plasmids and coexpression of the O:54 factor with other O-factors in different Salmonella serovars. The base composition of the pWQ799 replicon sequences gives an average percent G+C value typical of Salmonella spp. In contrast, the percent G+C value is dramatically lower with rfb0:54, consistent with the possibility that the cluster was acquired from an organism with much lower G+C composition.

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Year:  1995        PMID: 7545154      PMCID: PMC177315          DOI: 10.1128/jb.177.18.5247-5253.1995

Source DB:  PubMed          Journal:  J Bacteriol        ISSN: 0021-9193            Impact factor:   3.490


  61 in total

1.  Expression of antigenic factor O:54 is associated with the presence of a plasmid in Salmonella.

Authors:  M Y Popoff; L Le Minor
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2.  Methylation-dependent transcription controls plasmid replication of the CloDF13 cop-1(Ts) mutant.

Authors:  A J van Putten; R de Lang; E Veltkamp; H J Nijkamp; P Van Solingen; J A van den Berg
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3.  Control of ColE1 plasmid replication: binding of RNA I to RNA II and inhibition of primer formation.

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Review 4.  ColE1 replication control circuitry: sense from antisense.

Authors:  B Polisky
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Review 5.  The function of antibody and complement in the lysis of bacteria.

Authors:  M M Frank; K Joiner; C Hammer
Journal:  Rev Infect Dis       Date:  1987 Sep-Oct

6.  Characterization of the drug resistance plasmid NTP16.

Authors:  C M Lambert; C J Wrighton; P Strike
Journal:  Plasmid       Date:  1987-01       Impact factor: 3.466

7.  The complete nucleotide sequence of the bacteriocinogenic plasmid CloDF13.

Authors:  H J Nijkamp; R de Lang; A R Stuitje; P J van den Elzen; E Veltkamp; A J van Putten
Journal:  Plasmid       Date:  1986-09       Impact factor: 3.466

8.  Plasmid-encoded expression of lipopolysaccharide O-antigenic polysaccharide in enteropathogenic Escherichia coli.

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Authors:  D K Summers; D J Sherratt
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10.  Genesis of the novel epidemic Vibrio cholerae O139 strain: evidence for horizontal transfer of genes involved in polysaccharide synthesis.

Authors:  E M Bik; A E Bunschoten; R D Gouw; F R Mooi
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Authors:  Enrique D Vinés; Cristina L Marolda; Aran Balachandran; Miguel A Valvano
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Journal:  J Bacteriol       Date:  2001-01       Impact factor: 3.490

9.  Genetic analysis of the dTDP-rhamnose biosynthesis region of the Escherichia coli VW187 (O7:K1) rfb gene cluster: identification of functional homologs of rfbB and rfbA in the rff cluster and correct location of the rffE gene.

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Journal:  J Bacteriol       Date:  1995-10       Impact factor: 3.490

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