Hairy gene homolog increases nasopharyngeal carcinoma cell stemness by upregulating <i>Bmi-1</i>

Ye Lei; Hong-Fen Shen; Qi-Wen Li; Sheng Yang; Hong-Ting Xie; Xu-Feng Li; Mei-Ling Chen; Jia-Wei Xia; Sheng-Chun Wang; Guan-Qi Dai; Ying Zhou; Ying-Chun Li; Shi-Hao Huang; Dan-Hua He; Zhi-Hao Zhou; Jin-Ge Cong; Xiao-Lin Lin; Tao-Yan Lin; Ai-Bing Wu; Dong Xiao; Sheng-Jun Xiao; Xin-Ke Zhang; Jun-Shuang Jia

doi:doi:10.18632/aging.204742

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Research Paper Volume 15, Issue 10 pp 4391—4410

Hairy gene homolog increases nasopharyngeal carcinoma cell stemness by upregulating Bmi-1

Figure 3. RNAi-induced knockdown of Bmi-1 inhibited the in vitro proliferation and in vivo tumorigenesis of NPC cells. (A) The relative mRNA levels of Bmi-1 in shBmi-1-expressing 5-8F and SUNE1 cells were determined via qRT-PCR. SCR: scrambled control shRNA. (B) The protein levels of Bmi-1 in shBmi-1-expressing 5-8F and SUNE1 cells were determined via Western blotting. (C, D) A CCK8 assay was employed to assess the growth of shBmi-1-expressing 5-8F and SUNE1 cells. (E, F) A colony formation assay was used to examine the proliferation abilities of shBmi-1-expressing 5-8F and SUNE1 cells. (G, H) Propidium iodide staining and flow cytometry were used to detect the cell cycle distributions of shBmi-1-expressing 5-8F and SUNE1 cells (G), and the statistical results were calculated (H). (I–K) Bmi-1 knockdown inhibited tumor growth from 5-8F cells in nude mice. A representative tumor picture is shown (I), along with a tumor volume growth curve (J) and the tumor weights (K).