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Vol. 180, Issue 13, 3317-3322, July 1, 1998
Gene Replacement Analysis of the Streptomyces virginiae
barA Gene Encoding the Butyrolactone Autoregulator Receptor
Reveals that BarA Acts as a Repressor in Virginiamycin
Biosynthesis
Hiroko
Nakano,
Emio
Takehara,
Takuya
Nihira, and
Yasuhiro
Yamada
Department of Biotechnology, Graduate School
of Engineering, Osaka University, 2-1 Yamadaoka, Suita, Osaka 565, Japan
Virginiae butanolides (VBs), which are among the butyrolactone
autoregulators of Streptomyces species, act as a primary
signal in Streptomyces virginiae to trigger virginiamycin
biosynthesis and possess a specific binding protein, BarA. To clarify
the in vivo function of BarA in the VB-mediated signal pathway that
leads to virginiamycin biosynthesis, two barA
mutant strains (strains NH1 and NH2) were created by homologous
recombination. In strain NH1, an internal 99-bp EcoT14I
fragment of barA was deleted, resulting in an in-frame
deletion of 33 amino acid residues, including the second helix of
the probable helix-turn-helix DNA-binding motif. With the same growth
rate as wild-type S. virginiae on both solid and liquid
media, strain NH1 showed no apparent changes in its morphological behavior, indicating that the VB-BarA pathway does not
participate in morphological control in S. virginiae. In
contrast, virginiamycin production started 6 h earlier in strain
NH1 than in the wild-type strain, demonstrating for the first time that BarA is actively engaged in the control of virginiamycin production and
implying that BarA acts as a repressor in virginiamycin biosynthesis. In strain NH2, an internal EcoNI-SmaI fragment
of barA was replaced with a divergently oriented neomycin
resistance gene cassette, resulting in the C-terminally truncated BarA
retaining the intact helix-turn-helix motif. In strain NH2 and in a
plasmid-integrated strain containing both intact and mutated
barA genes, virginiamycin production was abolished
irrespective of the presence of VB, suggesting that the mutated BarA
retaining the intact DNA-binding motif was dominant over the wild-type
BarA. These results further support the hypothesis that BarA works as a
repressor in virginiamycin production and suggests that the
helix-turn-helix motif is essential to its function. In
strain NH1, VB production was also abolished, thus indicating that BarA
is a pleiotropic regulatory protein controlling not only
virginiamycin production but also autoregulator biosynthesis.
Copyright © 1998 by American Society for Microbiology
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