MicroRNA-182 regulates colon cancer cell proliferation and migration by targeting special AT-rich sequence-binding protein 2 gene

中华实验外科杂志 Pub Date : 2020-01-08 DOI:10.3760/CMA.J.ISSN.1001-9030.2020.01.018

Xu Jizhong, Gui-xian Wang, W. Yuan, Quanbo Zhou, Shengyun Hu

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Abstract

Objective To observe the effect of microRNA (miRNA, miR)-182 on the proliferation and migration of colorectal cancer cells by targeting special AT-rich sequence-binding protein 2 (SATB2) gene, and to explore its effect on SATB2/icotinamide adenine dinucleotide phosphate oxidase 4 (nox4) pathway. Methods HT-29 cells in logarithmic phase were transfected with Si-miR-182 and Control-si resectively, by liposome transfection, serving as Si-miR-182 group and N-miR-182 group, respectively. The expression of miR-182 gene, the cell proliferation and migration, the mRNA and protein expression of SATB2, nox4, E-cadherin and vimentin were examined. Results The relative expression of miR-182 gene in Si-miR-182 group (0.35±0.05) was lower than that in control group (1.24±0.26) and N-miR-182 group (1.20±0.25) (t=7.517, 7.455, P<0.05). The A values of methyl thiazol tetrazolium (MTT) test in Si-miR-182 group were lower than those in control group and N-miR-182 group after 24, 48 and 72 h of culture (24 h: t=2.667, 2.664; 48 h: t=4.559, 4.524; 72 h: t=7.257, 6.981; P<0.05). Compared with 24-h culture, the A value of MTT test in 48 and 72 hours in three groups were increased (48 h: t=5.507, 5.092, 3.741; 72 h: t=11.330, 10.637, 9.229; P<0.05), and the A value of MTT test in 72 hours were higher than those in 48 hours(t=7.411, 6.941, 5.214, P<0.05). The cell migration rate of Si-miR-182 group [(53.90±3.19)%] was lower than that of the control group [(81.66±5.92)%] and N-miR-182 group [(80.35±5.40)%] (t=9.231, 9.430, P<0.05). The relative expressions of SATB2, E-cadherin mRNA and protein in Si-miR-182 group were higher than those in control group and N-miR-182 group (SATB2: t=10.930, 11.158; E-Cadherin: t=9.288, 9.369; P<0.05), while the relative expressions of nox4, vimentin mRNA and protein in Si-miR-182 group were lower than those in control group and N-miR-182 group (nox4: t=8.955, 7.590; Vimentin: t=6.543, 6.644; P<0.05). Conclusion Silencing of miR-182 gene can significantly inhibit the proliferation and migration of colorectal cancer cells, possibly by activating SATB2, E-Cadherin expression, inhibiting the expression of nox4, Vimentin, and participating in the SATB2/nox4 pathway. Key words: MicroRNA-182; Special AT-rich sequence-binding protein 2; Colorectal cancer; Proliferation; Migration

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MicroRNA-182靶向特异性AT-富序列结合蛋白2基因调节结肠癌细胞增殖和迁移

目的观察microRNA (miRNA, miR)-182靶向特殊的富含at序列结合蛋白2 (SATB2)基因对结直肠癌细胞增殖和迁移的影响，并探讨其对SATB2/烟酰胺腺嘌呤二核苷酸磷酸氧化酶4 (nox4)通路的影响。方法脂质体转染对数期HT-29细胞Si-miR-182和Control-si，分别作为Si-miR-182组和N-miR-182组。检测miR-182基因表达、细胞增殖和迁移、SATB2、nox4、E-cadherin、vimentin mRNA和蛋白表达。结果Si-miR-182组miR-182基因相对表达量(0.35±0.05)低于对照组(1.24±0.26)和N-miR-182组(1.20±0.25)(t=7.517, 7.455, P<0.05)。培养24、48、72 h后，Si-miR-182组甲基噻唑四氮唑(MTT)检验A值均低于对照组和N-miR-182组(24 h: t=2.667、2.664;48 h: t=4.559, 4.524;72 h: t=7.257, 6.981;P < 0.05)。与24 h培养相比，3组小鼠48、72 h MTT试验A值均升高(48 h: t=5.507、5.092、3.741;72 h: t=11.330, 10.637, 9.229;P<0.05)，且72 h的MTT试验A值高于48 h (t=7.411、6.941、5.214,P<0.05)。Si-miR-182组细胞迁移率[(53.90±3.19)%]低于对照组[(81.66±5.92)%]和N-miR-182组[(80.35±5.40)%](t=9.231, 9.430, P<0.05)。Si-miR-182组SATB2、E-cadherin mRNA和蛋白的相对表达量均高于对照组和N-miR-182组(SATB2: t=10.930, 11.158;E-Cadherin: t=9.288, 9.369;P<0.05)，而Si-miR-182组nox4、vimentin mRNA和蛋白的相对表达量低于对照组和N-miR-182组(nox4: t=8.955, 7.590;Vimentin: t=6.543, 6.644;P < 0.05)。结论miR-182基因沉默可显著抑制结直肠癌细胞的增殖和迁移，其机制可能是激活SATB2、E-Cadherin的表达，抑制nox4、Vimentin的表达，参与SATB2/nox4通路。关键词:MicroRNA-182;特殊AT-rich序列结合蛋白2;结直肠癌;扩散;迁移

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