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Pleiotropic role of the Sco1/SenC family copper chaperone in the physiology of Streptomyces

Antibiotic production and cell differentiation in Streptomyces is stimulated by micromolar levels of Cu(2+). Here, we knocked out the Sco1/SenC family copper chaperone (ScoC) encoded in the conserved gene cluster ‘sco’ (the S treptomycescopper utilization) in Streptomyces coelicolor A3(2) and S. gri...

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Autores principales: Fujimoto, Masahiro, Yamada, Akio, Kurosawa, Junpei, Kawata, Akihiro, Beppu, Teruhiko, Takano, Hideaki, Ueda, Kenji
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Blackwell Publishing Ltd 2012
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3815325/
https://www.ncbi.nlm.nih.gov/pubmed/22117562
http://dx.doi.org/10.1111/j.1751-7915.2011.00319.x
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author Fujimoto, Masahiro
Yamada, Akio
Kurosawa, Junpei
Kawata, Akihiro
Beppu, Teruhiko
Takano, Hideaki
Ueda, Kenji
author_facet Fujimoto, Masahiro
Yamada, Akio
Kurosawa, Junpei
Kawata, Akihiro
Beppu, Teruhiko
Takano, Hideaki
Ueda, Kenji
author_sort Fujimoto, Masahiro
collection PubMed
description Antibiotic production and cell differentiation in Streptomyces is stimulated by micromolar levels of Cu(2+). Here, we knocked out the Sco1/SenC family copper chaperone (ScoC) encoded in the conserved gene cluster ‘sco’ (the S treptomycescopper utilization) in Streptomyces coelicolor A3(2) and S. griseus. It is known that the Sco1/SenC family incorporates Cu(2+) into the active centre of cytochrome oxidase (cox). The knockout caused a marked delay in antibiotic production and aerial mycelium formation on solid medium, temporal pH decline in glucose‐containing liquid medium, and significant reduction of cox activity in S. coelicolor. The scoC mutant produced two‐ to threefold higher cellular mass of the wild type exhibiting a marked cox activity in liquid medium supplied with 10 µM CuSO(4), suggesting that ScoC is involved in not only the construction but also the deactivation of cox. The scoC mutant was defective in the monoamine oxidase activity responsible for cell aggregation and sedimentation. These features were similarly observed with regard to the scoC mutant of S. griseus. The scoC mutant of S. griseus was also defective in the extracellular activity oxidizing N,N′‐dimethyl‐p‐phenylenediamine sulfate. Addition of 10 µM CuSO(4) repressed the activity of the conserved promoter preceding scoA and caused phenylalanine auxotrophy in some Streptomyces spp. probably because of the repression of pheA; pheA encodes prephenate dehydratase, which is located at the 3′ terminus of the putative operon structure. Overall, the evidence indicates that Sco is crucial for the utilization of copper under a low‐copper condition and for the activation of the multiple Cu(2+)‐containing oxidases that play divergent roles in the complex physiology of Streptomyces.
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spelling pubmed-38153252014-02-12 Pleiotropic role of the Sco1/SenC family copper chaperone in the physiology of Streptomyces Fujimoto, Masahiro Yamada, Akio Kurosawa, Junpei Kawata, Akihiro Beppu, Teruhiko Takano, Hideaki Ueda, Kenji Microb Biotechnol Research Articles Antibiotic production and cell differentiation in Streptomyces is stimulated by micromolar levels of Cu(2+). Here, we knocked out the Sco1/SenC family copper chaperone (ScoC) encoded in the conserved gene cluster ‘sco’ (the S treptomycescopper utilization) in Streptomyces coelicolor A3(2) and S. griseus. It is known that the Sco1/SenC family incorporates Cu(2+) into the active centre of cytochrome oxidase (cox). The knockout caused a marked delay in antibiotic production and aerial mycelium formation on solid medium, temporal pH decline in glucose‐containing liquid medium, and significant reduction of cox activity in S. coelicolor. The scoC mutant produced two‐ to threefold higher cellular mass of the wild type exhibiting a marked cox activity in liquid medium supplied with 10 µM CuSO(4), suggesting that ScoC is involved in not only the construction but also the deactivation of cox. The scoC mutant was defective in the monoamine oxidase activity responsible for cell aggregation and sedimentation. These features were similarly observed with regard to the scoC mutant of S. griseus. The scoC mutant of S. griseus was also defective in the extracellular activity oxidizing N,N′‐dimethyl‐p‐phenylenediamine sulfate. Addition of 10 µM CuSO(4) repressed the activity of the conserved promoter preceding scoA and caused phenylalanine auxotrophy in some Streptomyces spp. probably because of the repression of pheA; pheA encodes prephenate dehydratase, which is located at the 3′ terminus of the putative operon structure. Overall, the evidence indicates that Sco is crucial for the utilization of copper under a low‐copper condition and for the activation of the multiple Cu(2+)‐containing oxidases that play divergent roles in the complex physiology of Streptomyces. Blackwell Publishing Ltd 2012-07 2012-06-07 /pmc/articles/PMC3815325/ /pubmed/22117562 http://dx.doi.org/10.1111/j.1751-7915.2011.00319.x Text en Journal compilation © 2012 Society for Applied Microbiology and Blackwell Publishing Ltd
spellingShingle Research Articles
Fujimoto, Masahiro
Yamada, Akio
Kurosawa, Junpei
Kawata, Akihiro
Beppu, Teruhiko
Takano, Hideaki
Ueda, Kenji
Pleiotropic role of the Sco1/SenC family copper chaperone in the physiology of Streptomyces
title Pleiotropic role of the Sco1/SenC family copper chaperone in the physiology of Streptomyces
title_full Pleiotropic role of the Sco1/SenC family copper chaperone in the physiology of Streptomyces
title_fullStr Pleiotropic role of the Sco1/SenC family copper chaperone in the physiology of Streptomyces
title_full_unstemmed Pleiotropic role of the Sco1/SenC family copper chaperone in the physiology of Streptomyces
title_short Pleiotropic role of the Sco1/SenC family copper chaperone in the physiology of Streptomyces
title_sort pleiotropic role of the sco1/senc family copper chaperone in the physiology of streptomyces
topic Research Articles
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3815325/
https://www.ncbi.nlm.nih.gov/pubmed/22117562
http://dx.doi.org/10.1111/j.1751-7915.2011.00319.x
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