miR-let-7c-3p targeting on Egr-1 contributes to the committed differentiation of leukemia cells into monocyte/macrophages

被引:3
|
作者
Qi, Fu [1 ]
Wang, Xinping [2 ]
Zhao, Shouzhen [3 ]
Wang, Chaozhe [1 ]
Sun, Ruijing [1 ]
Wang, Huan [3 ]
Du, Pengchao [1 ]
Wang, Jing [4 ]
Wang, Xidi [5 ,6 ]
Jiang, Guosheng [1 ,3 ,7 ]
机构
[1] Binzhou Med Univ, Dept Immunol, Yantai 264000, Shandong, Peoples R China
[2] Yantai Hosp Tradit Chinese Med, Dept Lab Med, Yantai 264000, Shandong, Peoples R China
[3] Weifang Med Univ, Sch Life Sci & Technol, Weifang 261053, Shandong, Peoples R China
[4] Shandong Yinfeng Acad Life Sci, Dept Cellular Immunol, Jinan 250109, Shandong, Peoples R China
[5] Jining Med Univ, Lab Precis Med, Zhangqiu Dist Peoples Hosp Jinan, Jinan 250200, Shandong, Peoples R China
[6] Jining Med Univ, Lab Precis Med, Zhangqiu Dist Peoples Hosp Jinan, 1920 Huiquan Rd, Jinan 250200, Shandong, Peoples R China
[7] Binzhou Med Univ, Dept Immunol, 346 Guanhai Rd, Yantai 264000, Shandong, Peoples R China
基金
中国国家自然科学基金;
关键词
K562; cell; differentiation; microRNA-let-7c-3p; early growth response-1; macrophage; EARLY GROWTH RESPONSE-1; ACUTE MYELOID-LEUKEMIA; TRANSCRIPTION FACTOR; APOPTOSIS INDUCTION; UP-REGULATION; PROLIFERATION; EXPRESSION; CANCER;
D O I
10.3892/ol.2022.13393
中图分类号
R73 [肿瘤学];
学科分类号
100214 ;
摘要
In preliminary experiments, it was found that the expression of early growth response-1 (Egr-1) was upregulated during the committed differentiation of leukemia cells into monocytes/macrophages. The cross-analysis of gene chip detection and database prediction indicated that Egr-1 was associated with upstream microRNA (miR)-let-7c-3p, thus the present study focused on the role of the miR-let-7c-3p/Egr-1 signaling axis in the committed differentiation of leukemia cells into monocytes/macrophages. Phorbol 12-myristate 13-acetate (PMA) was used to induce the directed differentiation of human K562 leukemia cells into monocytes/macrophages and the differentiation of K562 leukemia cells was determined by cell morphology observation and expression of differentiation antigens CD11b and CD14 by flow cytometry. The expression levels of Egr-1 and miR-let-7c-3p were detected by reverse transcription-quantitative PCR and the protein expression of Egr-1 was detected by western blotting. The effect of Egr-1 on the differentiation of K562 cells was detected by short interfering (si)RNA interference assay. A dual-luciferase reporter assay was used to detect target binding of miR-let-7c-3p on the 3 ' UTR of Egr-1. Cell transfection of miR-let-7c-3p mimics and inhibitors was used to modulate the expression of miR-let-7c-3p, as indicated by RT-qPCR assays. Western blotting was also used to examine the effect of miR-let-7c-3p on Egr-1 expression. The PMA-induced differentiation of K562 cells was transfected with miR-let-7c-3p and the expression of differentiation antigen was detected by flow cytometry. A differentiation model of K562 leukemia cells into monocytes/macrophages was induced by PMA, which was indicated by morphological observations and upregulation of CD11b and CD14 antigens. The gene or protein expression of Egr-1 was significantly higher compared with that of the control group, while the expression of miR-let-7c-3p was significantly lower compared with that of the control group. siRNA interference experiments showed that the expression of cell differentiation antigen CD14 in the 100 mu g/ml PMA + si-Egr-1 group was significantly lower compared with that in the 100 mu g/ml PMA + si-ctrl group. The dual luciferase reporter gene results showed that the luciferase activity of the co-transfected mimic and Egr-1 WT groups was significantly lower than that of the NC control group, while the luciferase activity of the co-transfected mimic and Egr-1 MUT groups was comparable to that of the NC control group. Therefore, the dual-luciferase reporter gene assay confirmed that miR-let-7c-3p can target Egr-1. Western blotting showed that the expression of Egr-1 following transfection with miR-let-7c-3p inhibitor was significantly higher compared with that of the negative control and the expression of Egr-1 after transfection with miR-let-7c-3p mimic was significantly lower than that of the negative control. Following exposure to PMA, the expressions of CD11b and CD14 in the miR-let-7c-3p inhibitor group were significantly higher than those in the miR-let-7c-3p NC group, as indicated by CD11b and CD14 respectively. In conclusion, miR-let-7c-3p could bind to the 3 ' UTR of Egr-1 and negatively regulated Egr-1 expression. The miR-let-7c-3p/Egr-1 signaling axis was closely associated with the committed differentiation of K562 cells from leukemia cells to monocytes/macrophages.
引用
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页数:13
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