Publication | Open Access
Cloning and Heterologous Expression of the Grecocycline Biosynthetic Gene Cluster
69
Citations
45
References
2016
Year
Bioorganic ChemistryEntire Gene ClusterEngineeringMolecular BiologyChemical BiologyHeterologous ExpressionProtein SynthesisBiosynthesisThiol GroupGene StructureBiochemical GeneticsMetabolic EngineeringNatural Product BiosynthesisYeastMolecular BiotechnologyBiochemistryTransformation-associated RecombinationGene ExpressionBiomolecular EngineeringProtein BiosynthesisNatural SciencesSynthetic BiologyProtein Engineering
Transformation-associated recombination (TAR) in yeast is a rapid and inexpensive method for cloning and assembly of large DNA fragments, which relies on natural homologous recombination. Two vectors, based on p15a and F-factor replicons that can be maintained in yeast, E. coli and streptomycetes have been constructed. These vectors have been successfully employed for assembly of the grecocycline biosynthetic gene cluster from Streptomyces sp. Acta 1362. Fragments of the cluster were obtained by PCR and transformed together with the "capture" vector into the yeast cells, yielding a construct carrying the entire gene cluster. The obtained construct was heterologously expressed in S. albus J1074, yielding several grecocycline congeners. Grecocyclines have unique structural moieties such as a dissacharide side chain, an additional amino sugar at the C-5 position and a thiol group. Enzymes from this pathway may be used for the derivatization of known active angucyclines in order to improve their desired biological properties.
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