The long non-coding RNA TP73-AS1 modulates HCC cell proliferation through miR-200a-dependent HMGB1/RAGE regulation

被引:102
作者
Li, Shaling [1 ]
Huang, Yan [1 ]
Huang, Yun [2 ]
Fu, Yongming [1 ]
Tang, Daolin [3 ]
Kang, Rui [3 ]
Zhou, Rongrong [1 ]
Fan, Xue-gong [1 ]
机构
[1] Cent S Univ, Xiangya Hosp, Dept Infect Dis, Hunan Key Lab Viral Hepatitis, Changsha 410008, Hunan, Peoples R China
[2] Cent S Univ, Xiangya Hosp, Dept Surg, Changsha 410008, Hunan, Peoples R China
[3] Univ Pittsburgh, Dept Surg, Pittsburgh, PA 15260 USA
关键词
lncRNA; TP73-AS1; miR-200a; HCC; HMGB1; Proliferation; HUMAN HEPATOCELLULAR-CARCINOMA; TUMOR-GROWTH; CLINICOPATHOLOGICAL FEATURES; INCREASED EXPRESSION; TARGETING HMGB1; KIDNEY CANCER; PROGRESSION; SUPPRESSES; PROGNOSIS; MIGRATION;
D O I
10.1186/s13046-017-0519-z
中图分类号
R73 [肿瘤学];
学科分类号
100214 ;
摘要
Background: P73 antisense RNA 1 T ( non-protein coding), also known as TP73-AS1, is a long non-coding RNA (lncRNA) which is involved in cell proliferation and the development of tumors. However, the exact effects and molecular mechanisms of TP73-AS1 in hepatocellular carcinoma (HCC) progression are still unknown. The present study is aimed to investigate the detailed functions and the mechanism of TP73-AS1 in regulation of HCC cell proliferation. Methods: TP73-AS1 expression in HCC tissues and cell lines was determined using real-time PCR assays; the correlation of TP73-AS1 expression with clinicopathological features of HCC was analyzed. The functions of TP73-AS1 in regulation of HCC cell proliferation was evaluated using MTT and BrdU assays. The candidate upstream miRNAs of HMGB1 were screened using miRcode, miRWalk, miRanda and Target scan, verified using real-time PCR assays. The interaction between TP73-AS1 and miR-200a was confirmed using Luciferase report gene assays. The proten levels of HMGB1 signaling-related factors in response to co-processing TP73-AS1 knockdown and miR-200a inhibition were determined using Western blot assays and ELISA. Further, miR-200a, HMGB1 mRNA and RAGE mRNA and their correlations in HCC tissues were determined. Results: TP73-AS1 was upregulated in HCC tissues and cell lines. High TP73-AS1 expression was correlated with worse clinicopathological features, poorer prognosis and shorter survival. Knockdown of TP73-AS1 inhibited the HCC proliferation and the expression levels of HMGB1, RAGE and NF-kappa B in HCC cells. By using online tools, we screened out several candidate upstream miRNAs of HMGB1, among which miR-200a overexpression inhibited HMGB1 mRNA expression the most significantly. By using luciferase assays, we confirmed that miR-200a could directly bind to TP73-AS1 and the 3'UTR of HMGB1; TP73-AS1 competed with HMGB1 for miR-200a binding. MiR-200a inhibition could up-regulate HMGB1, RAGE, NF-kappa B expression as well as NF-kappa B regulated cytokines levels, which could be partially restored by si-TP73-AS1. In HCC tissues, miR-200a was down-regulated while HMGB1 and RAGE were up-regulated; TP73-AS1 was inversely correlated with miR-200a, while positively correlated with HMGB1 and RAGE, respectively. Conclusion: Our data indicated that TP73-AS1 might be an oncogenic lncRNA that promoted proliferation of HCC and could be regarded as a therapeutic target in human HCC.
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页数:12
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