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J. Bacteriol., 11 1995, 6069-6076, Vol 177, No. 21
B Perez-Esteban, E Gomez-Pardo and MA Penalva
Secondary metabolism, usually superfluous under laboratory conditions, is
intrinsically elusive to genetic analysis of its regulation. We describe
here a method of analyzing regulatory mutations affecting expression of
secondary metabolic genes, with an Aspergillus nidulans penicillin
structural gene (ipnA [encoding isopenicillin N-synthase]) as a model. The
method is based on a targeted double integration of a lacZ fusion reporter
gene in a chromosome different from that containing the penicillin gene
cluster. The trans-acting regulatory mutations simultaneously affect lacZ
expression and penicillin biosynthesis. One of these mutations (npeE1) has
been analyzed in detail. This mutation is recessive, prevents penicillin
production and ipnA'::'lacZ expression, and results in very low levels of
the ipnA message at certain times of growth. This indicates that npeE
positively controls ipnA transcription. We also show that this tandem
reporter fusion allows genetic analysis of npeE1 by using the sexual and
parasexual cycles and that lacZ expression is an easily scorable phenotype.
Haploidization analysis established that npeE is located in chromosome IV,
but npeE1 does not show meiotic linkage to a number of known chromosome IV
markers. This method might be of general applicability to genetic analysis
of regulation of other fungal secondary metabolic pathways.
Copyright © 1995, American Society for Microbiology
A lacZ reporter fusion method for the genetic analysis of regulatory mutations in pathways of fungal secondary metabolism and its application to the Aspergillus nidulans penicillin pathway
Departamento de Microbiologia Molecular, Centro de Investigaciones Biologicas del Consejo Superior de Investigaciones Cientificas, Madrid, Spain.
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