| 干扰LncRNA LRRC75A-AS1抑制肺癌细胞发生发展研究 |
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| 引用本文: | 吴迪,沈兆坤,陈聪.干扰LncRNA LRRC75A-AS1抑制肺癌细胞发生发展研究[J].蚌埠医学院学报,2022,47(4):442-446. |
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| 作者姓名: | 吴迪 沈兆坤 陈聪 |
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| 作者单位: | 盘锦辽油宝石花医院 心胸外科,辽宁 盘锦 124010 |
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| 摘 要: | 目的:探讨LncRNA LRRC75A-AS1/miR-22-3p对肺癌细胞增殖、凋亡、迁移的影响及其可能作用机制.方法:采用qRT-PCR法检测肺癌组织与癌旁组织中LRRC75A-AS1、miR-22-3p的表达水平;体外培养人肺癌细胞A549,si-NC、si-LRRC75A-AS1、si-LRRC75A-AS1与...
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| 关 键 词: | 肺肿瘤 LncRNA LRRC75A-AS1 miR-22-3p 增殖 凋亡 迁移 |
| 收稿时间: | 2021-03-26 |
Effect of Inhibition of LncRNA LRRC75 A-AS1 on the development of lung cancer cells |
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| WU Di,SHEN Zhao-kun,CHEN Cong.Effect of Inhibition of LncRNA LRRC75 A-AS1 on the development of lung cancer cells[J].Journal of Bengbu Medical College,2022,47(4):442-446. |
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| Authors: | WU Di SHEN Zhao-kun CHEN Cong |
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| Institution: | Department of Cardio-Thoracic Surgery, Panjin Liaoyou Baoshihua Hospital, Panjin Liaoning 124010, China |
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| Abstract: | ObjectiveTo explore the effect of LncRNA LRRC75A-AS1/miR-22-3p on the proliferation, apoptosis and migration in lung cancer cells.MethodsThe qRT-PCR method was used to detect the expressions of LRRC75A-AS1 and miR-22-3p in lung cancer tissues and adjacent tissues.Human lung cancer cells A549 were cultured in vitrol, si-NC, si-LRRC75A-AS1, si-LRRC75A-AS1 and anti-miR-NC, si-LRRC75A-AS1 and miR-22-3p inhibitor were transfected into A549 cells.The qRT-PCR method was used to detect the expressions of LRRC75A-AS1 and miR-22-3p in A549 cells.MTT assay and plate clone formation experiment were used to detect cell proliferation and clone formation ability, respectively.Flow cytometry was used to detect the apoptosis rate.Scratch test was used to detect cell migration ability.The dual luciferase reporter experiment was used to detect the targeting relationship between LRRC75A-AS1 and miR-22-3p.Western blotting was used to detect the expression of cleaved-caspase3 protein.ResultsCompared with adjacent tissues, the expression of LRRC75A-AS1 in lung cancer tissues was increased (1.01±0.13) vs(4.59±0.34)](P < 0.01), and the expression level of miR-22-3p was decreased (1.00±0.12)vs(0.28±0.04)](P < 0.01).Compared with the si-NC group, the cell survival rate of the si-LRRC75A-AS1 group was reduced100%vs(54.45±2.21)%](P < 0.01), the number of clone formation was reduced(121.00±5.10) vs(58.67±2.49)](P < 0.01), the apoptosis rate was increased(8.42±0.34)%vs(25.59±0.80)%](P < 0.01), the protein level of cleaved-caspase3 was increased (0.20±0.01)vs(0.68±0.05)](P < 0.01), and the rate of scratch healing was decreased (66.71±1.43)%vs(32.56±0.95)%](P < 0.01).The dual luciferase report experiment confirmed that LRRC75A-AS1 could act as a competitive endogenous RNA for miR-22-3p.Compared with the si-LRRC75A-AS1+anti-miR-NC group, the cell survival rate of the si-LRRC75A-AS1+miR-22-3p inhibitor group was increased(54.61±2.28)%vs(88.75±3.22)%](P < 0.01), the number of clones was increased (57.67±2.49)vs(106.67±3.68)](P < 0.01), the apoptosis rate was decreased (25.63±0.99)%vs(13.11±0.55)%](P < 0.01), the scratch healing rate was increased (32.52±0.98)%vs(55.30±1.18)%](P < 0.01), and the protein level of cleaved-caspase3 was decreased(0.67±0.06)vs(0.30±0.03)](P < 0.01).ConclusionsInhibiting the expression of LRRC75A-AS1 may reduce the proliferation, migration and clone formation ability of lung cancer cells by up-regulating miR-22-3p, which can induce cell apoptosis. |
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