| Article ID | Journal | Published Year | Pages | File Type |
|---|---|---|---|---|
| 1393740 | Chemistry & Biology | 2012 | 9 Pages |
SummaryTerpendole E is the first natural product inhibitor of kinesin Eg5. Because terpendole E production is unstable, we isolated and analyzed the terpendole E biosynthetic gene cluster, which consists of seven genes encoding three P450 monooxygenases (TerP, TerQ, and TerK), an FAD-dependent monooxygenase (TerM), a terpene cyclase (TerB), and two prenyltransferases (TerC and TerF). Gene knockout and feeding experiments revealed that terpendole E is a key intermediate in terpendole biosynthesis and is produced by the action of the key enzyme TerQ from paspaline, a common biosynthetic intermediate of indole-diterpenes. TerP converts terpendole E to a downstream intermediate specific to terpendole biosynthesis and converts paspaline to shunt metabolites. We successfully overproduced terpendole E by disrupting the terP gene. We propose that terpendole E is a key biosynthetic intermediate of terpendoles and related indole-diterpenes.
Graphical AbstractFigure optionsDownload full-size imageDownload high-quality image (212 K)Download as PowerPoint slideHighlights► The terpendole biosynthetic gene cluster was isolated ► Terpendole E is a key biosynthetic intermediate of indole-diterpenes ► Terpendole E was overproduced by gene knockout of the bispecific enzyme TerP ► Indole-diterpene biosynthetic pathways can be classified into two groups
