Polyketide Synthase Genes from Marine Dinoflagellates

: AbstractRapidly developing techniques for manipulating the pathways of polyketide biosynthesis at the genomic level have created the demand for new pathways with novel biosynthetic capability. Polyketides derived from dinoflagellates are among the most complex and unique structures identified thus...

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Published inMarine biotechnology (New York, N.Y.) Vol. 5; no. 1; pp. 1 - 12
Main Authors Snyder, R V, Gibbs, P D L, Palacios, A, Abiy, L, Dickey, R, Lopez, J V, Rein, K S
Format Journal Article
LanguageEnglish
Published United States Springer-Verlag 01.01.2003
Springer Nature B.V
Subjects
Animals
Bacteria
Biosynthesis
Cloning
Dinoflagellida - enzymology
Dinoflagellida - genetics
Dinophyta
DNA - isolation & purification
Enzymes
Gene Expression Profiling
Genes
Genetic Testing
Gymnodinium catenatum
Laboratories
Marine biology
Multienzyme Complexes - genetics
Polyketide synthase
Polymerase chain reaction
Proteins
Reverse Transcriptase Polymerase Chain Reaction
RNA - isolation & purification
rRNA 16S
saxitoxin
Seafood
Sequence Analysis, DNA
Species Specificity
Studies
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Summary:: AbstractRapidly developing techniques for manipulating the pathways of polyketide biosynthesis at the genomic level have created the demand for new pathways with novel biosynthetic capability. Polyketides derived from dinoflagellates are among the most complex and unique structures identified thus far, yet no studies of the biosynthesis of dinoflagellate-derived polyketides at the genomic level have been reported. Nine strains representing 7 different species of dinoflagellates were screened for the presence of type I and type II polyketide synthases (PKSs) by polymerase chain reaction (PCR) and reverse transcriptase PCR. Seven of the 9 strains yielded products that were homologous with known and putative type I PKSs. Unexpectedly, a PKS gene was amplified from cultures of the dinoflagellate Gymnodinium catenatum, a saxitoxin producer, which is not known to produce a polyketide. In each case the presence of a PKS gene was correlated with the presence of bacteria in the cultures as identified by amplification of the bacterial 16S ribosomal RNA gene. However, amplification from polyadenylated RNA, the lack of PKS expression in light-deprived cultures, residual phylogenetic signals, resistance to methylation-sensitive restriction enzymes, and the lack of hybridization to bacterial isolates support a dinoflagellate origin for most of these genes.
Bibliography:http://dx.doi.org/10.1007/s10126-002-0077-y
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ISSN:1436-2228
1436-2236
DOI:10.1007/s10126-002-0077-y