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J. Bacteriol., 11 1995, 6246-6254, Vol 177, No. 21
GH Feng and TJ Leonard
Aflatoxins are potent toxic and carcinogenic compounds, produced by
Aspergillus parasiticus and A. flavus as secondary metabolites. In this
research, a polyketide synthase gene (pksL1), the key gene for aflatoxin
biosynthesis initiation in A. parasiticus, has been functionally identified
and molecularly characterized. PCR-derived DNA probes were used to find the
pksL1 gene from subtracted, aflatoxin- related clones. Gene knockout
experiments generated four pksL1 disruptants which lost both the ability to
produce aflatoxins B1, B2, and G1 and the ability to accumulate
norsolorinic acid and all other intermediates of the aflatoxin biosynthetic
pathway. A pksL1 DNA probe detected a 6.6-kb poly(A)+ RNA transcript in
Northern (RNA) hybridizations. This transcript, associated with aflatoxin
production, exhibited a regulated expression that was influenced by growth
phase, medium composition, and culture temperature. DNA sequencing of pksL1
revealed an open reading frame for a polypeptide (PKSL1) of 2,109 amino
acids. Sequence analysis further recognized four functional domains in
PKSL1, acyl carrier protein, beta-ketoacyl-acyl carrier protein synthase,
acyltransferase, and thioesterase, all of which are usually present in
polyketide synthases and fatty acid synthases. On the basis of these
results, we propose that pksL1 encodes the polyketide synthase which
synthesizes the backbone polyketide and initiates aflatoxin biosynthesis.
In addition, the transcript of pksL1 exhibited heterogeneity at the
polyadenylation site similar to that of plant genes.
Copyright © 1995, American Society for Microbiology
Characterization of the polyketide synthase gene (pksL1) required for aflatoxin biosynthesis in Aspergillus parasiticus
Department of Genetics, University of Wisconsin, Madison 53706, USA.
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