Development of platensimycin, platencin, and platensilin overproducers by biosynthetic pathway engineering and fermentation medium optimization

Lucas L Fluegel; Ming-Rong Deng; Ping Su; Edward Kalkreuter; Dong Yang; Jeffrey D Rudolf; Liao-Bin Dong; Ben Shen

doi:10.1093/jimb/kuae003

Development of platensimycin, platencin, and platensilin overproducers by biosynthetic pathway engineering and fermentation medium optimization

J Ind Microbiol Biotechnol. 2024 Jan 9:51:kuae003. doi: 10.1093/jimb/kuae003.

Authors

Lucas L Fluegel^{1

2}, Ming-Rong Deng¹, Ping Su¹, Edward Kalkreuter¹, Dong Yang^{1

3}, Jeffrey D Rudolf¹, Liao-Bin Dong¹, Ben Shen^{1

2

3

4}

Affiliations

¹ D epartment of Chemistry, The Herbert Wertheim UF Scripps Institute for Biomedical Innovation & Technology, University of Florida, Jupiter, FL 33458, USA.
² Skaggs Graduate School of Chemical and Biological Sciences, Scripps Research, Jupiter, FL 33458, USA.
³ Natural Products Discovery Center, The Herbert Wertheim UF Scripps Institute for Biomedical Innovation & Technology, University of Florida, Jupiter, FL 33458, USA.
⁴ Department of Molecular Medicine, The Herbert Wertheim UF Scripps Institute for Biomedical Innovation & Technology, University of Florida, Jupiter, FL 33458, USA.

Abstract

The platensimycin (PTM), platencin (PTN), and platensilin (PTL) family of natural products continues to inspire the discovery of new chemistry, enzymology, and medicine. Engineered production of this emerging family of natural products, however, remains laborious due to the lack of practical systems to manipulate their biosynthesis in the native-producing Streptomyces platensis species. Here we report solving this technology gap by implementing a CRISPR-Cas9 system in S. platensis CB00739 to develop an expedient method to manipulate the PTM, PTN, and PTL biosynthetic machinery in vivo. We showcase the utility of this technology by constructing designer recombinant strains S. platensis SB12051, SB12052, and SB12053, which, upon fermentation in the optimized PTM-MS medium, produced PTM, PTN, and PTL with the highest titers at 836 mg L-1, 791 mg L-1, and 40 mg L-1, respectively. Comparative analysis of these resultant recombinant strains also revealed distinct chemistries, catalyzed by PtmT1 and PtmT3, two diterpene synthases that nature has evolved for PTM, PTN, and PTL biosynthesis. The ΔptmR1/ΔptmT1/ΔptmT3 triple mutant strain S. platensis SB12054 could be envisaged as a platform strain to engineer diterpenoid biosynthesis by introducing varying ent-copalyl diphosphate-acting diterpene synthases, taking advantage of its clean metabolite background, ability to support diterpene biosynthesis in high titers, and the promiscuous tailoring biosynthetic machinery.

One-sentence summary: Implementation of a CRISPR-Cas9 system in Streptomyces platensis CB00739 enabled the construction of a suite of designer recombinant strains for the overproduction of platensimycin, platencin, and platensilin, discovery of new diterpene synthase chemistries, and development of platform strains for future diterpenoid biosynthesis engineering.

Keywords: Biosynthesis; Medium optimization; Pathway engineering; Platencin; Platensilin; Platensimycin.

MeSH terms

Adamantane*
Aminobenzoates*
Aminophenols*
Anilides*
Biological Products*
Biosynthetic Pathways
Diterpenes* / metabolism
Fermentation
Polycyclic Compounds*
Streptomyces*

Substances

platencin
platensimycin
Diterpenes
Biological Products
Aminophenols
Aminobenzoates
Polycyclic Compounds
Adamantane
Anilides

Supplementary concepts

Streptomyces platensis

Abstract

MeSH terms

Substances

Supplementary concepts

Grants and funding