Molecular profiling of ginsenoside metabolites to identify estrogen receptor alpha activity

Mami Kikegawa; Azusa Nakajima; Jing Yu; Masashi Asai; Yoshihiro Uesawa; Hideko Sone

doi:10.1016/j.gene.2021.146108

Molecular profiling of ginsenoside metabolites to identify estrogen receptor alpha activity

Gene. 2022 Mar 1:813:146108. doi: 10.1016/j.gene.2021.146108. Epub 2021 Dec 18.

Authors

Mami Kikegawa¹, Azusa Nakajima², Jing Yu², Masashi Asai², Yoshihiro Uesawa³, Hideko Sone⁴

Affiliations

¹ Department of Kampo Medicine, Yokohama University of Pharmacy, Yokohama 245-0066, Japan; Department of Medical Molecular Informatics, Meiji Pharmaceutical University, Tokyo 204-8588, Japan.
² Department of Kampo Medicine, Yokohama University of Pharmacy, Yokohama 245-0066, Japan.
³ Department of Medical Molecular Informatics, Meiji Pharmaceutical University, Tokyo 204-8588, Japan.
⁴ Department of Kampo Medicine, Yokohama University of Pharmacy, Yokohama 245-0066, Japan. Electronic address: hideko.sone@yok.hamayaku.ac.jp.

PMID: 34929341
DOI: 10.1016/j.gene.2021.146108

Abstract

20(S)-Protopanaxadiol (PPD) and 20(S)-Protopanaxatriol (PPT) are major metabolites of ginseng in humans and are considered to have estrogenic activity in cellular bioassays. In this study, we conducted in silico analyses to determine whether PPD and PPT interact with estrogen receptor alpha (ERα) and compared them with ERα agonists, partial agonists, and antagonists to identify their ERα activity. The transcriptome profile of 17β-estradiol (E2), PPD, and PPT in MCF-7 cells expressing ERα was further compared to understand the ERα activity of ginsenoside metabolites. The results showed that PPD and PPT interacted with the 1ERE, 1GWR, and 3UUD ERα proteins in the E2 interaction model, the 3ERD protein in the diethylstilbestrol (DES) interaction model, and the 1X7R protein in the genistein (GEN) interaction model. Conversely, neither the 4PP6 protein of the interaction model with the antagonist resveratrol (RES) nor the 1ERR protein of the interaction model with the antagonist raloxifene (RAL) showed the conformation of amino acid residues. When E2, PPD, and PPT were exposed to MCF-7 cells, cell proliferation and gene expression were observed. The transcriptomic profiles of E2, PPD, and PPT were compared using a knowledge-based pathway. PPD-induced transcription profiling was similar to that of E2, and the neural transmission pathway was detected in both compounds. In contrast, PPT-induced transcription profiling displayed characteristics of gene expression associated with systemic lupus erythematosus. These results suggest that ginsenoside metabolites have ERα agonist activity and exhibit neuroprotective effects and anti-inflammatory actions. However, a meta-analysis using public microarray data showed that the mother compounds GRb1 and GRg1 of PPD and PPT showed metabolic functions in insulin signaling pathways, condensed DNA repair and cell cycle pathways, and immune response and synaptogenesis. These results suggest that the ginsenoside metabolites have potent ERα agonist activity; however, their gene expression profiles may differ from those of E2.

Keywords: 20(S)-Protopanaxadiol; 20(S)-Protopanaxatriol; Estrogen Receptor Alpha Activity; Ginsenoside Metabolites; Molecular Docking.

MeSH terms

Cell Proliferation / drug effects
Estradiol / pharmacology
Estrogen Receptor alpha / genetics
Estrogen Receptor alpha / metabolism*
Estrogen Receptor beta / genetics
Gene Expression
Genistein / pharmacology
Ginsenosides / genetics
Ginsenosides / metabolism
Humans
MCF-7 Cells
Molecular Docking Simulation / methods
Resveratrol / pharmacology
Sapogenins / metabolism*
Sapogenins / pharmacology
Signal Transduction / drug effects
Transcriptome
Triterpenes / metabolism*
Triterpenes / pharmacology

Substances

ESR1 protein, human
Estrogen Receptor alpha
Estrogen Receptor beta
Ginsenosides
Sapogenins
Triterpenes
protopanaxtriol
Estradiol
Genistein
protopanaxadiol
Resveratrol