[Cloning of transcription factor PcFBA-1 in Pogostemon cabin and its interaction with FPPS promoter]

Hui-Ling Huang; Dai-di Wu; Dan-Hua Zhang; Xi-Lin Wang; Jie-Xuan Zhuang; Ruo-Ting Zhan; Li-Kai Chen

doi:10.19540/j.cnki.cjcmm.20211026.101

[Cloning of transcription factor PcFBA-1 in Pogostemon cabin and its interaction with FPPS promoter]

Zhongguo Zhong Yao Za Zhi. 2022 Jan;47(2):412-418. doi: 10.19540/j.cnki.cjcmm.20211026.101.

[Article in Chinese]

Authors

Hui-Ling Huang¹, Dai-di Wu¹, Dan-Hua Zhang¹, Xi-Lin Wang¹, Jie-Xuan Zhuang¹, Ruo-Ting Zhan², Li-Kai Chen²

Affiliations

¹ School of Chinese Materia Medica, Guangzhou University of Chinese Medicine Guangzhou 510006, China Key Laboratory of Chinese Medicinal Resource from Lingnan, Ministry of Education, Guangzhou University of Chinese Medicine Guangzhou 510006, China.
² School of Chinese Materia Medica, Guangzhou University of Chinese Medicine Guangzhou 510006, China Key Laboratory of Chinese Medicinal Resource from Lingnan, Ministry of Education, Guangzhou University of Chinese Medicine Guangzhou 510006, China Maoming Branch, Guangdong Laboratory for Lingnan Modern Agriculture Maoming 525000, China.

PMID: 35178983
DOI: 10.19540/j.cnki.cjcmm.20211026.101

Abstract

Farnesyl diphosphate synthase(FPPS) is a key enzyme at the branch point of the sesquiterpene biosynthetic pathway, but there are no reports on the transcriptional regulation of FPPS promoter in Pogostemon cabin. In the early stage of this study, we obtained the binding protein PcFBA-1 of FPPS gene promoter in P. cabin. In order to explore the possible mechanism of PcFBA-1 involved in the regulation of patchouli alcohol biosynthesis, this study performed PCR-based cloning and sequencing analysis of PcFBA-1, analyzed the expression patterns of PcFBA-1 in different tissues by fluorescence quantitative PCR and its subcellular localization using the protoplast transformation system, detected the binding of PcFBA-1 protein to the FPPS promoter in vitro with the yeast one-hybrid system, and verified its transcriptional regulatory function by dual-luciferase reporter gene assay. The findings demonstrated that the cloned PcFBA-1 had an open reading frame(ORF) of 1 131 bp, encoding a protein of 376 amino acids, containing two conserved domains named F-box-like superfamily and FBA-1 superfamily, and belonging to the F-box family. Moreover, neither signal peptide nor transmembrane domain was contained, implying that it was an unstable hydrophilic protein. In addition, as revealed by fluorescence quantitative PCR results, PcFBA-1 had the highest expression in leaves, and there was no significant difference in expression in roots or stems. PcFBA-1 protein was proved mainly located in the cytoplasm. Furthermore, yeast one-hybrid screening and dual-luciferase reporter gene assay showed that PcFBA-1 was able to bind to FPPS promoter both in vitro and in vivo to enhance the activity of FPPS promoter. In summary, this study identifies a new transcription factor PcFBA-1 in P. cabin, which directly binds to the FPPS gene promoter to enhance the promoter activity. This had laid a foundation for the biosynthesis of patchouli alcohol and other active ingre-dients and provided a basis for metabolic engineering and genetic improvement of P. cabin.

Keywords: FPPS; Pogostemon cabin; promoter; protein-DNA interaction; transcriptional regulation.

MeSH terms

Amino Acid Sequence
Cloning, Molecular
Geranyltranstransferase / genetics
Pogostemon*
Transcription Factors / genetics

Substances

Transcription Factors
Geranyltranstransferase