5HRE增强子和hTERT启动子联合调控CDX2基因对人结肠癌细胞系LoVo增殖的抑制  被引量:4

Effects of a hypoxia-induced,tumor-specific gene therapy vector on proliferation of human colon carcinoma cell line LoVo Human colon adenocarcinoma cell line

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作  者:贺赛[1] 郑见宝[1] 孙学军[1] 陈南征[1] 周培华[1] 魏光兵[1] 王晖[1] 姚建锋[1] 张立[1] 贾蓬勃[1] 

机构地区:[1]西安交通大学医学院第一附属医院普通外科,陕西西安710061

出  处:《中国肿瘤生物治疗杂志》2014年第3期314-319,共6页Chinese Journal of Cancer Biotherapy

基  金:国家自然科学基金资助项目(No.81101874;No.81172362;No.81172359);陕西省科学技术研究发展计划项目(No.2011-K12-19);陕西省科技统筹创新工程计划项目(No.2013KTCQ03-08)~~

摘  要:目的:检测已构建的缺氧反应元件(hypoxia response element,HRE)和人端粒酶催化亚单位(human telomerase reverse transcriptase,hTERT)启动子调控CDX2基因表达的载体pLVX-5HRE-hTERTp-CDX2-3FLAG(5HhC)对人结肠癌细胞系LoVo增殖的影响。方法:复苏前期筛选的转染pLVX-hTERTp-CDX2-3FLAG(hC)的LoVo细胞(hC/LoVo)、转染pLVX-5HREhTERTp-3FLAG(5Hh)的LoVo细胞(5Hh/LoVo)、转染pLVX-5HRE-hTERTp-CDX2-3FLAG(5HhC)的LoVo细胞(5HhC/LoVo)及空白LoVo细胞,各组细胞均在常氧条件和缺氧条件(加入缺氧模拟剂CoCl2)展开实验。MTT检测细胞增殖情况,平板克隆实验观察细胞集落形成,流式细胞术分析细胞周期。结果:成功复苏转染5HhC的LoVo细胞及各组对照LoVo细胞。hC/LoVo、5HhC/LoVo细胞增殖显著低于LoVo及5Hh/LoVo,且缺氧微环境下的5HhC对于LoVo细胞的增殖速度抑制更为明显[细胞增殖率,第5天,常氧vs缺氧:(48.62±3.32)%vs(36.81±2.83)%,P<0.05;第7天,常氧vs缺氧:(56.44±2.28)%vs(38.51±3.21)%,P<0.05]。hC/LoVo、5HhC/LoVo组的平板克隆数显著低于LoVo及5Hh/LoVo组,且缺氧微环境下的5HhC对LoVo细胞集落形成能力的抑制较常氧环境下更为显著[集落数:(44.2±3.5)个vs(90.8±9.3)个,P<0.05];hC/LoVo、5HhC/LoVo组G1期细胞比例较LoVo细胞及5Hh/LoVo组明显提高[(63.59±0.55)%、(64.82±2.22)%vs(51.38±0.70)%、(51.59±0.38)%,P<0.05],且在缺氧微环境下,5HhC/LoVo组G1期细胞比例提高更加显著[(71.38±3.02)%vs(64.82±2.22)%,P<0.05]。结论:治疗载体5HhC可使人结肠癌细胞系LoVo发生G1期阻滞,增殖及集落形成能力受到抑制,且在缺氧诱导下5HhC的抑制能力更为显著。Objective: Homebox transcription factor 2( CDX2) has been described as a colorectal tumor suppressor. This study aimed to evaluate the effect of overexpression of the hypoxia response element enhancer( HRE) sequence-inserted CDX2 gene under the control of the human telomerase reverse transcriptase( hTERT) promoter on proliferation of human colon adenocarcinoma LoVo cells in vitro. Methods: Stable clones of LoVo cells expressing pLVX-hTERTp-CDX2-3FLAG( hC),pLVX-5HRE-hTERTp-3FLAG( 5Hh) and pLVX-5HRE-hTERTp-CDX2-3FLAG( 5HhC),respectively, were generated. LoVo cells stably expressing hC,5Hh,and 5HhC,respectively,were cultured under hypoxia control( CoCl 2 200 μmol / L) and normoxia,respectively. At the designated time points of culture,cell viability was assessed by MTT assays,colony-forming capacity by trypan blue staining and cell cycle progression by flow cytometry. Result: Viability was significantly decreased in hC-and 5HhC-expressing LoVo cells as compared with wild-type LoVo cells and 5Hh-expressing LoVo cells. The proliferation rates under normoxia and hypoxiarespectively were( 48. 62 ± 3. 32) % and( 36.81 ±2. 83) % at 5 days( P 〈0.05) and( 56.44 ±2. 28) % and( 38. 51 ±3. 21) % at 7 days( P 〈0.05) in 5HhCexpressing cells. LoVo cells stably expressing hC and 5HhC,respectively,formed significantly less clones than cells stably expressing 5Hhunder a hypoxic condition( 44. 2 ± 3. 5 vs 90. 8 ± 9. 3,P 〈 0. 05). The proportion of cells at G 1 phase arrest was( 63. 59 ± 0. 55) % and( 64. 82 ± 2. 22) % in cells stably expressing hC and 5HhC respectively,significantly higher( P 〈 0. 05) than that in wild type LoVo cells and cells stably expression 5Hh( 51. 38 ± 0. 70 and 51. 59 ± 0. 38) under normoxia. Under a hypoxic condition,as high as 71. 38 ± 3. 02 5HhC-expressing LoVo cells were arrested at G 1 phase. Conclusion: Overexpression of the CDX2 gene carrying the HRE sequence driven by the hTERT promoter may significantl

关 键 词:基因治疗 结肠癌 缺氧 CDX2基因 细胞增殖 

分 类 号:R735.35[医药卫生—肿瘤] R730.59[医药卫生—临床医学]

 

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