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      Characterization of the iron-regulated desA promoter of Streptomyces pilosus as a system for controlled gene expression in actinomycetes

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      1 , 2 , 1 , 2 ,
      Microbial Cell Factories
      BioMed Central

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          Abstract

          Background

          The bioavailability of iron is quite low since it is usually present as insoluble complexes. To solve the bioavailability problem microorganisms have developed highly efficient iron-scavenging systems based on the synthesis of siderophores that have high iron affinity. The systems of iron assimilation in microorganisms are strictly regulated to control the intracellular iron levels since at high concentrations iron is toxic for cells. Streptomyces pilosus synthesizes the siderofore desferrioxamine B. The first step in desferrioxamine biosynthesis is decarboxylation of L-lysine to form cadaverine, a desferrioxamine B precursor. This reaction is catalyzed by the lysine decarboxylase, an enzyme encoded by the desA gene that is repressed by iron.

          Results

          The binding of the DmdR (acronym for divalent metal dependent repressor) to the desA promoter in presence of Fe 2+ or other divalent ions has been characterized. A 51 bp DNA fragment of the desA promoter containing the 9 bp inverted repeat was sufficient for binding of the DmdR repressor, as observed by the electrophoretic mobility shift assay. The desA mobility shift was prevented by neutralizing DmdR with anti-DmdR antibodies or by chelating the divalent metal in the binding reaction with 2,2'-dipyridyl. Binding to the desA promoter was observed with purified DmdR repressors of Streptomyces coelicolor or Rhodococcus fascians suggesting that there is a common mechanism of iron-regulation in actinomycetes. The complete desA promoter region was coupled using transcriptional fusions to the amy reporter gene (encoding α-amylase) in low copy or multicopy Streptomyces vectors. The iron-regulated desA promoter was induced by addition of the iron chelating agent 2,2'-dipyridyl resulting in a strong expression of the reporter gene.

          Conclusions

          The iron-regulated desA promoter can be used for inducible expression of genes in Streptomyces species, as shown by de-repression of the promoter when coupled to a reporter gene.

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          Most cited references37

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          Siderophores: structure and function of microbial iron transport compounds.

          Siderophores are common products of aerobic and facultative anaerobic bacteria and of fungi. Elucidation of the molecular genetics of siderophore synthesis, and the regulation of this process by iron, has been facilitated by the fact that E. coli uses its own siderophores as well as those derived from other species, including fungi. Overproduction of the siderophore and its transport system at low iron is in this species well established to be the result of negative transcriptional repression, but the detailed mechanism may be positive in other organisms. Siderophores are transported across the double membrane envelope of E. coli via a gating mechanism linking the inner and outer membranes.
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            Microbial envelope proteins related to iron.

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              • Record: found
              • Abstract: not found
              • Article: not found

              Iron transport and storage.

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                Author and article information

                Journal
                Microb Cell Fact
                Microbial Cell Factories
                BioMed Central (London )
                1475-2859
                2003
                19 May 2003
                : 2
                : 5
                Affiliations
                [1 ]Area de Microbiología, Facultad de Ciencias Biológicas y Ambientales, Universidad de León, 24071 León, Spain
                [2 ]Institute of Biotechnology INBIOTEC, Science Park of León, Avda. del Real, n° 1, 24006 León, Spain
                Article
                1475-2859-2-5
                10.1186/1475-2859-2-5
                161790
                12801423
                f2e70b34-89a1-436a-a94f-803b6921656c
                Copyright © 2003 Flores et al; licensee BioMed Central Ltd. This is an Open Access article: verbatim copying and redistribution of this article are permitted in all media for any purpose, provided this notice is preserved along with the article's original URL.
                History
                : 9 April 2003
                : 19 May 2003
                Categories
                Research

                Biotechnology
                Biotechnology

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