| STC-1蛋白对肾癌细胞生长平衡影响机制探讨 |
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| 引用本文: | 杨清滔,;谷江,;张永春,;杨永安,;王楠,;朱致晖,;祝庆亮.STC-1蛋白对肾癌细胞生长平衡影响机制探讨[J].肿瘤防治杂志,2014(14):1078-1083. |
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| 作者姓名: | 杨清滔 ;谷江 ;张永春 ;杨永安 ;王楠 ;朱致晖 ;祝庆亮 |
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| 作者单位: | [1]贵阳医学院附属医院泌尿外科,贵州贵阳550004; [2]江都人民医院泌尿外科,江苏扬州225200 |
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| 基金项目: | 贵州省科技厅社会攻关计划[黔科合sy字(2011)3060] |
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| 摘 要: | 目的:研究斯钙素1(stanniocalcin1,STC-1)与缺氧诱导因子1α(hypoxia-inducible factor 1α,HIF-1α)的相互作用,是否借助调节Ca2+水平参与肾癌细胞生长调控。方法:构建高表达HIF-1α的肾癌细胞模型,使用不同浓度STC-1蛋白干预转染后的肾癌细胞(转染组)和单纯肾癌细胞(非转染组)。MTT法检测各组细胞增殖情况;RT-PCR及ELISA法检测细胞内HIF-1α、STC-1基因及蛋白表达;荧光分光光度计检测细胞内Ca2+水平。结果:非转染组和转染组肾癌细胞HIF-1α蛋白表达分别为8.3±1.2和15.1±0.9,t=24.18,P〈0.001;STC-1蛋白表达分别为7.2±0.9和10.8±1.1,t=8.90,P=0.003;提示转染HIF-1α的肾癌细胞内HIF-1α和STC-1表达显著提高。不同浓度STC-1溶液干预非转染组肾癌细胞24h后,对照组HIF-1α蛋白表达为8.3±0.5,低剂量组为7.8±0.7,中剂量组为5.3±0.4,高剂量组为4.2±0.3,F=171.726,P〈0.001,对照组STC-1蛋白表达为7.1±0.4,低剂量组为6.8±0.3,中剂量组为4.1±0.2,高剂量组为3.3±0.4,F=257.174,P〈0.001;对照组细胞内Ca2+含量为95.7±8.6,低剂量组为60.3±5.5,中剂量组为48.6±6.3,高剂量组为33.7±4.2,F=198.931,P〈0.001,对照组细胞增殖活性为0.226±0.021,低剂量组为0.343±0.024,中剂量组为0.293±0.018,高剂量组为0.252±0.023,F=23.615,P〈0.001;不同浓度STC-1溶液干预转染组肾癌细胞24h后,对照组HIF-1α蛋白表达为15.3±1.6,低剂量组为14.6±1.1,中剂量组为10.1±0.9,高剂量组为8.6±0.8,F=135.696,P〈0.001,对照组STC-1蛋白表达为11.2±0.4,低剂量组为10.9±0.5,中剂量组为7.4±0.7,高剂量组为5.6±0.8,F=105.101,P〈0.001;对照组细胞内Ca2+含量为65.5±6.7,低剂量组为40.1±3.4,中剂量组为30.7±4.6,高剂量组为17.7±3.3,F=136.621,P〈0.001;对照组细胞增殖活性为0.295±0.033,低剂量组为0.446±0.025,中剂量组为0.379±0.015,高剂量组为0.313±0.022,F=45.571,P〈0.001。提示STC-1蛋白可促进单纯肾癌细胞和转染后肾癌?
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| 关 键 词: | 肾癌细胞 斯钙素1 缺氧诱导因子1α 钙离子 细胞增殖 抑制 |
Influence of STC-1 and HIF-1α on growth balance in renal carcinoma cells |
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| Institution: | YANG Qing-tao ,GU Jiang ,ZHANG Yong-chun ,YANG Yong-an ,WANG Nan , ZHU Zhi-hui , ZHU Qing-liang (1. Department of Urologic Surgery ,Affiliated Hospital ,Guiyang Medical College ,Guiyang 550004 ,P. R. China 2. Department of Urologic Surgery, Jiangdu People's Hospital ,Yangzhou 225200, P. R. China) |
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| Abstract: | OBJECTIVE: To research the regulation of proliferation and discuss whether Stanniocalcinl (STC-1), Hypoxia-inducible factor 1α (HIF-1α) and Ca2+ were participated in proliferation mechanism of renal carcinoma cells. METHODS: After successfully constructed the HIF-I~ highly expressing cell models, different concentrations of STC-1 solutions were added to the culture medium, then, proliferation of cells, expressions of HIF-la, STC-1 and levels of Ca2+ were detected by MTT, RT-PCR, ELISA and Fluorescence Speetrophotometer respectively. RESULTS: HIF-1α protein ex pression in non-transfected group and transferred group cells were 8.3 ± 1.2 and 15.1±0.9 respectively (t = 24. 18, P〈 0. 001). STC-1 protein expression in non-transfeeted group and transferred group cells were 7.2 ± 0. 9 and 10.8 ± 1. 1 respectively (t= 8.90, P= 0. 003). The results showed stable transfection of HIF-1α/pcDNA3.0 into renal carcinoma cells resulted in efficiently rised expression of HIF 1α and STC-1. Non-transfected group cells were exposed with STC-1 solutions of different concentration (0,0.1,0.5 and 1.0 nmol/L) for 24 hours,the expression of HIF-1α was 8.3±0.5,7.8± 0. 7,5. 3±0. 4 and 4.2±0.3 (F=171. 726,P〈0. 001) ,the expression of STC-1 was 7.1±0.4,6.8±0.3,4. 1±0.2 and 3.3±0.4 (F=257.174,P〈0.001),the levels of Ca2+ was 95.7±8.6,60.3±5.5,48.6±6.3 and 33.7±4.2 (F= 198. 931,P〈0. 001),the cells proliferative activity was 0. 226±0. 021,0. 343±0. 024,0. 293±0. 018 and 0. 252±0. 023 respectively (F= 23. 615,P〈0. 001). Transfected group ceils were exposed with STC-1 solutions of different concentra- tion (0,0.1,0.5 and 1.0 nmol/L) for 24 hours,the expression of HIF-la was 15.3±1.6,14.6±1.1,10.1±0.9 and 8.6±0.8 (F=135. 696,P〈0. 001) ,the expression of STC-1 was 11.2±0.4,10.9±0.5,7.4±0.7 and 5.6±0.8 (F= 105. 101,P〈0. 001) ,the levels of Ca2+ was 65.5±6.7,40.1±3.4,30.7±4.6 and 17.7±3.3 (F=136. 621,P〈0. 001), the cells proliferativ |
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| Keywords: | renal carcinoma cells stanniocalcinl hypoxia-inducible factor 1α calcium cell proliferation suppressor |
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