Study on the Effects of Deoxyschizandrin on the Proliferation ，Migration and Invasion of Human Nasopharyngeal Carcinoma Cell HONE- 1 via Met/PI 3K/Akt Signaling Pathway

Tengxiang Chen; Li Liang; Zhirui Zeng; Shan Lei; Jingya Wang; Yuanmei Sun; Jinzhi Lan; Yan Xue

Return

Study on the Effects of Deoxyschizandrin on the Proliferation ，Migration and Invasion of Human Nasopharyngeal Carcinoma Cell HONE- 1 via Met/PI 3K/Akt Signaling Pathway

VernacularTitle:基于Met/PI3K/Akt信号通路研究五味子甲素对人鼻咽癌细胞HONE-1增殖、迁移和侵袭的影响
Author: Tengxiang CHEN ^{1
,

2} ; Li LIANG ^{1
,

2} ; Zhirui ZENG ^{1
,

2} ; Shan LEI ^{1
,

2} ; Jingya WANG ^{1
,

2} ; Yuanmei SUN ^{1
,

2} ; Jinzhi LAN ^{2
,

3} ; Yan XUE ¹
Author Information

1. Dept. of Physiology，School of Basic Medical Sciences，Guizhou Medical University，Guiyang 550025，China
2. Guizhou Provincial Key Laboratory of Pathogenesis & Drug Research on Common Chronic Diseases，Guiyang 550025，China
3. Tissue Engineering and Stem Cell Research Center，Guizhou Medical University，Guiyang 550025，China
Publication Type:Journal Article
Keywords: Deoxyschizandrin; Proliferation; Migration
From: China Pharmacy 2020;31(19):2376-2381
CountryChina
Language:Chinese
Abstract: OBJECTIVE：To study the effects and potential mechani sm of deoxyschizandrin on the proliferation ，migration and invasion of nasopharyngeal carcinoma cell HONE- 1. METHODS ：HONE-1 cell was set as cell model ，while CCK- 8 test，wound healing assay and Transwell chamber test were used to detect the proliferation ，migration and invasion ability changes of HONE- 1 cells after treatment with different concentrations [ 0（blank control ），10，20，40 μmol/L] of deoxyschizandrin. Computer molecular docking was performed to analyze the binding ability between deoxyschizandrin and Met protein. Western blotting assay was used to detect the relative protein expressions of p-Met ，p-PI3K，p-Akt，Bcl-2 and N-cadherin in cells. RESULTS ：Compared with blank control ，the proliferation ，migration and invasion ability of cells after treated with 10，20，40 μmol/L deoxyschizandrin were all decreased significantly （P＜0.05）. Results of molecular docking revealed that deoxyschizandrin could stably bind with the activity pocket of Met protein. Results of Western blotting assay demonstrated that compared with blank control ，10，20，40 μmol/L deoxyschizandrin all decreased the relative protein expressions of p-Met ，p-PI3K，p-Akt，Bcl-2 and N-cadherin in cells significantly（P＜0.05）. CONCLUSIONS ：Deoxyschizandrin can inhibit the proliferation ，migration and invasion of HONE- 1 cell via inhibiting the activation of Met/PI 3K/Akt signaling pathway.