Nanomicellar TGX221 Inhibits N-Myc to Suppress Malignant Biological Behavior of Prostate Cancer Cells by Regulating MYC/Myc-Associated Factor X (MAX)

Author:

Li Hongwei1,Xu Lei2,Li Ming2,Gao Zhan3

Affiliation:

1. Department of Pathology, Zibo Central Hospital, Zibo, 255020, Shandong Province, China

2. Department of Urology, Zibo Central Hospital, Zibo, 255020, Shandong Province, China

3. Department of Clinical Laboratory, Zibo Central Hospital, 255020, Shandong Province, China

Abstract

Considering free amino N-terminal-myelocytomatosis viral oncogene homolog (N-Myc) as an important gene in prostate cancer (PC), we herein detected the impact of TGX-221 nanomicelles on N-Myc expression in PC cells. PC cells (LNCaP) were divided into blank group, empty vector group, N-Myc group and vector+N-Myc group, followed by analysis of myelocytomatosis viral oncogene homolog (MYC) and myc-associated factor (XMAX) expressions, cell proliferation, apoptosis and migration by CCK-8 method, flow cytometry and transwell experiment. Compared with blank group (4.95±0.67), N-Myc expression in the N-Myc group increased (6.25±0.78) but expressions in the empty vector (1.03±0.23) and vector+N-Myc groups (3.46±0.37) decreased significantly (P <0.05), with lowest expression in the empty vector group (P <0.05). Cell proliferation and migration in the N-Myc group increased within 96 h of transfection, but decreased in the empty vector and vector+N-Myc groups (P <0.05), and TGX-221-loaded N-Myc obtained the lowest proliferation and migration (P <0.05). N-Myc transfection decreased apoptosis, and nanomicellar TGX221 or N-Myc-loaded vector resulted in increased apoptotic cells (P < 0.05), with highest apoptosis in the vector+N-Myc group. Moreover, the presence of nanomicellar TGX221 reversed their expression with lowest expression in the vector+N-Myc group, as transfection with N-Myc increased MYC/MAX mRNA expression. TGX-221 nanomicelles inhibited N-Myc and MYC/MAX expression, thereby suppressing proliferation and migration of PC cells, and inducing cell apoptosis.

Publisher

American Scientific Publishers

Subject

Pharmaceutical Science,General Materials Science,Biomedical Engineering,Medicine (miscellaneous),Bioengineering

Reference52 articles.

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