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Heterologous expression of tylosin polyketide synthase and production of a hybrid bioactive macrolide in Streptomyces venezuelae
Authors:Won Seok Jung  Sang Kil Lee  Jay Sung Joong Hong  Sung Ryeol Park  Soon Jeong Jeong  Ah Reum Han  Jae Kyung Sohng  Byung Gee Kim  Cha Yong Choi  David H Sherman  Yeo Joon Yoon
Institution:(1) Interdisciplinary Program of Biochemical Engineering and Biotechnology, Seoul National University, San 56-1, Shilim-dong, Gwanak-gu, Seoul, 151-742, South Korea;(2) School of Chemical and Biological Engineering, Seoul National University, San 56-1, Shilim-dong, Gwanak-gu, Seoul, 151-742, South Korea;(3) Division of Nano Sciences, Department of Chemistry, Ewha Woman’s University, 11-1 Daehyun-dong, Seodaemun-gu, Seoul, 120-750, South Korea;(4) Institute of Biomolecule Reconstruction, Department of Pharmaceutical Engineering, Sun Moon University, Kalsan-ri, Tangjeong-myeon, Asan-si, Chungnam, 336-708, South Korea;(5) Life Sciences Institute, Department of Medicinal Chemistry, University of Michigan, 210 Washtenaw Avenue, Ann Arbor, MI 48109-2216, USA
Abstract:Tylosin polyketide synthase (Tyl PKS) was heterologously expressed in an engineered strain of Streptomyces venezuelae bearing a deletion of pikromycin PKS gene cluster using two compatible low-copy plasmids, each under the control of a pikAI promoter. The mutant strain produced 0.5 mg/l of the 16-membered ring macrolactone, tylactone, after a 4-day culture, which is a considerably reduced culture period to reach the maximum production level compared to other Streptomyces hosts. To improve the production level of tylactone, several precursors for ethylmalonyl-CoA were fed to the growing medium, leading to a 2.8-fold improvement (1.4 mg/ml); however, switching the pikAI promoter to an actI promoter had no observable effect. In addition, a small amount of desosamine-glycosylated tylactone was detected from the extract of the mutant strain, revealing that the native glycosyltransferase DesVII displayed relaxed substrate specificity in accepting the 16-membered ring macrolactone to produce the glycosylated tylactone. These results demonstrate a successful attempt for a heterologous expression of Tyl PKS in S. venezuelae and introduce S. venezuelae as a rapid heterologous expression system for the production of secondary metabolites.
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