Metabolic engineering of Saccharomyces cerevisiae for the biosynthesis of a fungal pigment from the phytopathogenic fungus Cladosporium phlei

Yeji Gwon; Kum-Kang So; Jeesun Chun; Dae-Hyuk Kim

doi:10.1186/s13036-024-00429-0

Metabolic engineering of Saccharomyces cerevisiae for the biosynthesis of a fungal pigment from the phytopathogenic fungus Cladosporium phlei

J Biol Eng. 2024 May 13;18(1):33. doi: 10.1186/s13036-024-00429-0.

Authors

Yeji Gwon^#¹, Kum-Kang So^#^{2

3}, Jeesun Chun^#^{2

3}, Dae-Hyuk Kim^{4

5

6}

Affiliations

¹ Department of Bioactive Material Sciences, Jeonbuk National University, Jeonju, 54896, Republic of Korea.
² Institute for Molecular Biology and Genetics, Jeonbuk National University, Jeonju, 54896, Republic of Korea.
³ Department of Molecular Biology, Jeonbuk National University, Jeonju, 54896, Republic of Korea.
⁴ Department of Bioactive Material Sciences, Jeonbuk National University, Jeonju, 54896, Republic of Korea. dhkim@jbnu.ac.kr.
⁵ Institute for Molecular Biology and Genetics, Jeonbuk National University, Jeonju, 54896, Republic of Korea. dhkim@jbnu.ac.kr.
⁶ Department of Molecular Biology, Jeonbuk National University, Jeonju, 54896, Republic of Korea. dhkim@jbnu.ac.kr.

^# Contributed equally.

Abstract

Background: Cladosporium phlei is a phytopathogenic fungus that produces a pigment called phleichrome. This fungal perylenequinone plays an important role in the production of a photosensitizer that is a necessary component of photodynamic therapy. We applied synthetic biology to produce phleichrome using Saccharomyces cerevisiae.

Results: The gene Cppks1, which encodes a non-reducing polyketide synthase (NR-PKS) responsible for the biosynthesis of phleichrome in C. phlei, was cloned into a yeast episomal vector and used to transform S. cerevisiae. In addition, a gene encoding a phosphopantetheinyl transferase (PPTase) of Aspergillus nidulans was cloned into a yeast integrative vector and also introduced into S. cerevisiae for the enzymatic activation of the protein product of Cppks1. Co-transformed yeasts were screened on a leucine/uracil-deficient selective medium and the presence of both integrative as well as episomal recombinant plasmids in the yeast were confirmed by colony PCR. The episomal vector for Cppks1 expression was so dramatically unstable during cultivation that most cells lost their episomal vector rapidly in nonselective media. This loss was also observed to a less degree in selective media. This data strongly suggests that the presence of the Cppks1 gene exerts a significant detrimental effect on the growth of transformed yeast cells and that selection pressure is required to maintain the Cppks1-expressing vector. The co-transformants on the selective medium showed the distinctive changes in pigmentation after a period of prolonged cultivation at 20 °C and 25 °C, but not at 30 °C. Furthermore, thin layer chromatography (TLC) revealed the presence of a spot corresponding with the purified phleichrome in the extract from the cells of the co-transformants. Liquid chromatography (LC/MS/MS) verified that the newly expressed pigment was indeed phleichrome.

Conclusion: Our results indicate that metabolic engineering by multiple gene expression is possible and capable of producing fungal pigment phleichrome in S. cerevisiae. This result adds to our understanding of the characteristics of fungal PKS genes, which exhibit complex structures and diverse biological activities.

Keywords: Cladosporium phlei; Saccharomyces cerevisiae; Phleichrome; Polyketide synthase.

Abstract

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