Effects of Bmi-1-siRNA on proliferation of lung adenocarcinoma SPC-A1 cells and its mechanism

王艺芳; 刘奔; 刘纯青; 郑翔宇; 刘丹丹; 朱杰; 杨春辉; 孟秀香

doi:10.3969/j.issn.1007-3969.2014.05.003

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Effects of Bmi-1-siRNA on proliferation of lung adenocarcinoma SPC-A1 cells and its mechanism

更新时间：2025-12-31

- Effects of Bmi-1-siRNA on proliferation of lung adenocarcinoma SPC-A1 cells and its mechanism
- China Oncology Vol. 24, Issue 5, Pages: 333-341(2014)
- 作者机构：
  
  1. 河南省红十字血液中心检验科,河南,郑州,450012
  2. 大连医科大学检验医学院,辽宁,大连,116044
  3. 大连医科大学诊断学实验中心,辽宁,大连,116044
  4. 大连医科大学第二临床学院检验科,辽宁,大连,116027
- 作者简介：
- 基金信息：
- DOI：10.3969/j.issn.1007-3969.2014.05.003
  CLC：
- Published Online：26 May 2014，
  
  Published：26 May 2014
- 稿件说明：
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王艺芳,刘奔,刘纯青,郑翔宇,刘丹丹,朱杰,杨春辉,孟秀香. Bmi-1-siRNA抑制肺腺癌SPC-A1细胞的增殖及其机制[J]. 中国癌症杂志, 2014, 24(5): 333-341.

王艺芳, 刘奔, 刘纯青, et al. Effects of Bmi-1-siRNA on proliferation of lung adenocarcinoma SPC-A1 cells and its mechanism[J]. China Oncology, 2014, 24(5): 333-341.
王艺芳,刘奔,刘纯青,郑翔宇,刘丹丹,朱杰,杨春辉,孟秀香. Bmi-1-siRNA抑制肺腺癌SPC-A1细胞的增殖及其机制[J]. 中国癌症杂志, 2014, 24(5): 333-341. DOI： 10.3969/j.issn.1007-3969.2014.05.003.

王艺芳, 刘奔, 刘纯青, et al. Effects of Bmi-1-siRNA on proliferation of lung adenocarcinoma SPC-A1 cells and its mechanism[J]. China Oncology, 2014, 24(5): 333-341. DOI： 10.3969/j.issn.1007-3969.2014.05.003.

摘要

背景与目的：Bmi-1(B-cell specific moloneymurine leukemiavirus insertion site 1)基因是多梳基因家族的重要成员之一，主要通过调控INK4a/ARF位点来调节细胞的增殖和衰老。本研究旨在探讨Bmi-1-siRNA对具有INK4a/ARF位点的肺腺癌SPC-A1细胞生长和增殖的影响，并探讨其作用机制。方法：①本实验选用已确定有效的siRNA序列进行病毒包装，构建反转录病毒si-Bmi-1 pSUPERretro-neo，然后感染到SPC-A1细胞中，建立稳定表达Bmi-1-siRNA的肺癌细胞株。②利用RT-PCR和蛋白质印迹法(Western blot)技术分析Bmi-1基因在Bmi-1-siRNA转染后SPC-A1细胞中表达情况。③利用台盼蓝拒染法、MTT法、平板克隆形成实验和裸鼠实验，分析Bmi-1-siRNA对SPC-A1细胞体内外增殖能力的影响。④利用流式细胞术分析SPC-A1各组细胞的周期分布。⑤利用Western blot法分析增殖通路相关分子：p16

INK4a

、p53、Cyclin D1、PTEN和Ser473p-Akt等蛋白表达情况。结果：反转录病毒介导的Bmi-1-siRNA被转染后，有效抑制了SPC-A1细胞中Bmi-1基因的转录和表达，抑制了SPC-A1细胞的体内外增殖能力(P0.01)，并使转染组细胞阻滞在G

期［(64.6±1.2)%，P0.05］。沉默Bmi-1基因后，与对照组细胞相比，p16

INK4a

、p53和Akt蛋白表达水平无明显变化(P0.05)，Cyclin D1和Ser473p-Akt表达水平下降(P0.01)，PTEN表达水平上调(P0.01)。用PTEN抑制剂处理转染组细胞后，Bmi-1和Ser473p-Akt蛋白表达得以重塑。结论：Bmi-1-siRNA通过将肺腺癌SPC-A1细胞周期阻滞于G

期来抑制肿瘤细胞增殖，这种抑制作用可能不依赖于p16

INK4a

来调控Cyclin D1的表达，进而参与调控肿瘤细胞增殖。

Abstract

Background and purpose: The human oncogene B-cell-specific moloney murine leukemia virus integration site 1 (Bmi-1) is an important member of the polycomb group family

and it regulates cell proliferation and senescence via INK4a/ARF locus. This study investigated the effects of Bm

i-1-siRNA on the proliferation of lung adenocarcinoma cell line SPC-A1 cells with INK4a/ARF locus and clarify the mechanism of Bmi-1-mediated effect on proliferation of lung adenocarcinoma cells. Methods: In this study

we chose the most efficient siRNA chain the pGeneshl-2-Bmi-1 sense-1 and inserted into a pSUPER-retro-neo retroviral vector. The packaged si-Bmi-1 pSUPERretro-neo retroviral vector was stably transfected into lung adenocarcinoma SPC-A1 cell line. The stably transfected cells were cultured and passed. After transfection

the levels of Bmi-1 mRNA and protein expression of SPC-A1 cells were analyzed by RT-PCR and Western blot respectively. Trypan blue

MTT and plate colony forming assay were performed to observe the proliferation capibility of SPC-A1 cells and evaluate the cloning forming ability in vitro. The potency of tumorigenesis was observed in nude mouse through hypodermic inoculation of SPC-A1 cells. Cell cycle distribution was analyzed by flow cytometry (FCM) in SPC-A1 cells. The expression levels of proliferation proteins including p16

INK4a

p53

Cyclin D1

PTEN

Akt and Ser473p-Akt were analyzed by Western blot. Results: The mRNA and protein expression levels of Bmi-1 were significantly reduced in SPC-A1-Bmi-1-siRNA cells transfected with pSUPER-retroneo retroviral vector. Knockdown of Bmi-1 could inhibit the growth

colony formation in vitro and tumorigenesis invivo of SPC-A1 cells (P0.01). The transfected SPC-A1 cells were arrested in G

phase ［(64.6±1.2)%

P0.05］.Compared with two control groups

p16

INK4a

p53 and Akt were not affected (P0.05)

while Cyclin D1 and Ser473p-Akt were downregulated (P0.01) and PTEN was up-regulated (P0.01) in the SPC-A1-Bmi-1-siRNA cells. SPC-A1-Bmi-1-siRNA cells were treated with various concentrations of PTEN inhibitor to determine expression levels of PTEN

Bmi-1 and Ser473p-Akt protein. Ablation of PTEN rescued Bmi-1 and Ser473p-Akt expression in SPC-A1-Bmi-1-siRNA cells. Conclusion: Knockdown of Bmi-1 gene can arrest the

proliferation of SPC-A1 cells through G

phasearrest by inhibiting Cyclin D1 expression indirectly

which may be not associated with p16

INK4a

signaling pathway.

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