Novel lncRNA PSMG3‑AS1 functions as a miR‑143‑3p sponge to increase the proliferation and migration of breast cancer cells

Yue Cui; Yuhua Fan; Guangcai Zhao; Qibing Zhang; Ying Bao; Yuanri Cui; Zengjie Ye; Guoyou Chen; Xianji Piao; Fang Guo; Jinghao Wang; Yuhua Bai; Dejun Yu

doi:10.3892/or.2019.7390

Novel lncRNA PSMG3‑AS1 functions as a miR‑143‑3p sponge to increase the proliferation and migration of breast cancer cells

Oncol Rep. 2020 Jan;43(1):229-239. doi: 10.3892/or.2019.7390. Epub 2019 Oct 25.

Authors

Yue Cui^#¹, Yuhua Fan^#², Guangcai Zhao¹, Qibing Zhang³, Ying Bao¹, Yuanri Cui³, Zengjie Ye⁴, Guoyou Chen², Xianji Piao¹, Fang Guo¹, Jinghao Wang⁵, Yuhua Bai², Dejun Yu¹

Affiliations

¹ Central Laboratory of The Fifth Affiliated Hospital of Harbin Medical University, Daqing, Heilongjiang 163711, P.R. China.
² Department of Pathology, Harbin Medical University, Daqing, Heilongjiang 163319, P.R. China.
³ Department of Breast Surgery of Daqing Oilfield General Hospital, Daqing, Heilongjiang 163001, P.R. China.
⁴ School of Nursing, Guangzhou University of Chinese Medicine, Guangzhou, Guangdong 510006, P.R. China.
⁵ Department of Pharmacy, The First Affiliated Hospital, Jinan University, Guangzhou, Guangdong 510006, P.R. China.

^# Contributed equally.

Abstract

Long non‑coding RNAs (lncRNAs) are considered to be important regulators in breast cancer. In the present study, the potential mechanisms and functional roles of lncRNA PSMG3‑antisense (AS)1 were investigated in vivo and in vitro. The relative expression levels of lncRNA PSMG3‑AS1 and microRNA (miR)‑143‑3p were determined using reverse‑transcription quantitative PCR. The protein expression levels of collagen type 1 alpha 1 (COL1A1) and proliferating cell nuclear antigen (PCNA) were obtained using western blot analysis. Bioinformatics analysis was used to identify the relationship between PSMG3‑AS1, miR‑143‑3p and COL1A1. Colony forming and Cell Counting Kit‑8 assays were used to detect cell proliferation. Transwell and wound‑healing assays were used to determine cell migration. The results of the present study demonstrated that PSMG3‑AS1 expression was increased in breast cancer tumor tissues and cell lines, and that of miR‑143‑3p was decreased. Knockdown of PSMG3‑AS1 increased the level of miR‑143‑3p expression, which led to the mitigation of proliferation and migration capacity in breast carcinoma cells. Additionally, PSMG3‑AS1 knockdown was demonstrated to reduce the mRNA and protein expression levels of COL1A1. miR‑143‑3p mimic transfection reduced proliferation and migration in MDA‑MB‑231 and MCF‑7 cell lines. Furthermore, miR‑143‑3p inhibition significantly increased the proliferation and migration of breast cancer cells compared with the negative control group. The mRNA and protein expression levels of PCNA were reduced in the MCF‑7 cell line when transfected with miR‑143‑3p mimics and si‑PSMG3‑AS1. However, PCNA expression was increased in cells transfected with a miR‑143‑3p inhibitor. In conclusion, the results of the present study identified a novel lncRNA PSMG3‑AS1, which serves as a sponge for miR‑143‑3p in the pathogenesis of breast cancer. PSMG3‑AS1 may be used as a potential therapeutic target gene in breast cancer treatment.

Keywords: breast cancer; PSMG3-AS1; miR-143-3p; COL1A1; proliferation; migration.

MeSH terms

Adult
Aged
Aged, 80 and over
Breast Neoplasms / genetics*
Breast Neoplasms / metabolism
Cell Line, Tumor
Cell Movement
Cell Proliferation
Collagen Type I / genetics*
Collagen Type I / metabolism*
Collagen Type I, alpha 1 Chain
Female
Gene Expression Regulation, Neoplastic
Gene Regulatory Networks
Humans
MCF-7 Cells
MicroRNAs / genetics*
Middle Aged
RNA, Long Noncoding / genetics*
Up-Regulation*

Substances

Collagen Type I
Collagen Type I, alpha 1 Chain
MIRN143 microRNA, human
MicroRNAs
RNA, Long Noncoding