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J. Bacteriol., 05 1995, 2892-2900, Vol 177, No. 10
W Margolin, D Bramhill and SR Long
Rhizobium meliloti exists either as a free-living soil organism or as a
differentiated endosymbiont bacteroid form within the nodules of its host
plant, alfalfa (Medicago sativa), where it fixes atmospheric N2.
Differentiation is accompanied by major changes in DNA replication and cell
division. In addition, R. meliloti harbors three unique large circular
chromosome-like elements whose replication coordination may be complex. As
part of a study of DNA replication control in R. meliloti, we isolated a
dnaA homolog. The deduced open reading frame predicts a protein of 57 kDa
that is 36% identical to the DnaA protein of Escherichia coli, and the
predicted protein was confirmed by immunoblot analysis. In a comparison
with the other known DnaA proteins, this protein showed the highest
similarity to that of Caulobacter crescentus and was divergent in some
domains that are highly conserved in other unrelated species. The dnaA
genes of a diverse group of bacteria are adjacent to a common set of genes.
Surprisingly, analysis of the DNA sequence flanking dnaA revealed none of
these genes, except for an rpsT homolog, also found upstream of dnaA in C.
crescentus. Instead, upstream of rpsT lie homologs of fpg, encoding a DNA
glycosylase, and fadB1, encoding an enoyl-coenzyme A hydratase with a
strikingly high (53 to 55%) level of predicted amino acid identity to two
mammalian mitochondrial homologs. Downstream of dnaA, there are two open
reading frames that are probably expressed but are not highly similar to
any genes in the databases. These results show that R. meliloti dnaA is
located within a novel gene arrangement.
Copyright © 1995, American Society for Microbiology
The dnaA gene of Rhizobium meliloti lies within an unusual gene arrangement
Department of Biological Sciences, Stanford University, California 94305-5020, USA.
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