natural biocombinatorics in the polyketide synthase genes of the actinobacterium streptomyces avermitilis自然biocombinatorics酮化合物合酶基因的actinobacterium链霉菌属avermitilis.pdfVIP

natural biocombinatorics in the polyketide synthase genes of the actinobacterium streptomyces avermitilis自然biocombinatorics酮化合物合酶基因的actinobacterium链霉菌属avermitilis.pdf

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natural biocombinatorics in the polyketide synthase genes of the actinobacterium streptomyces avermitilis自然biocombinatorics酮化合物合酶基因的actinobacterium链霉菌属avermitilis

Natural Biocombinatorics in the Polyketide Synthase Genes of the Actinobacterium Streptomyces avermitilis 1 ¨ 2 1* Holger Jenke-Kodama , Thomas Borner , Elke Dittmann 1 Department of Molecular Ecology, Institute of Biology, Humboldt University, Berlin, Germany, 2 Department of Genetics, Institute of Biology, Humboldt University, Berlin, Germany Modular polyketide synthases (PKSs) of bacteria provide an enormous reservoir of natural chemical diversity. Studying natural biocombinatorics may aid in the development of concepts for experimental design of genes for the biosynthesis of new bioactive compounds. Here we address the question of how the modularity of biosynthetic enzymes and the prevalence of multiple gene clusters in Streptomyces drive the evolution of metabolic diversity. The phylogeny of ketosynthase (KS) domains of Streptomyces PKSs revealed that the majority of modules involved in the biosynthesis of a single compound evolved by duplication of a single ancestor module. Using Streptomyces avermitilis as a model organism, we have reconstructed the evolutionary relationships of different domain types. This analysis suggests that 65% of the modules were altered by recombinational replacements that occurred within and between biosynthetic gene clusters. The natural reprogramming of the biosynthetic pathways was unambiguously confined to domains that account for the structural diversity of the polyketide products and never observed for the KS domains. We provide examples for natural acyltransferase (AT), ketoreductase (KR), and dehydratase (DH)–KR domain replacements. Potential sites of homologous recombination could be identified in interdomain regions and within domains. Our results indicate that homologous recombination facilitated by the modula

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