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论文摘要

2000年与2010年四川大学华西医院收治肺癌患者的临床流行病学特征及病理类型分布特点

Clinical Epidemiology and Histological Characteristics of Patients with Lung Cancer in West China Hospital of

作者:姚晓军, 张洪伟, 蒲强等

Author:YAO Xiao-jun, ZHNAG Hong-wei, PU Qiang. et al

收稿日期:          年卷(期)页码:2014,45(2):309-315

期刊名称:四川大学学报(医学版)

Journal Name:JOURNAL OF SICHUAN UNIVERSITY (MEDICAL SCIENCE EDITION)

关键字:肺肿瘤 流行病学 病理学

Key words:Lung neoplasms Epidemiology Pathology

基金项目:

中文摘要

目的 回顾性分析四川大学华西医院2000年与2010年收治的原发性支气管肺癌患者的临床流行病学特征及病理类型分布,以初步了解肺癌的流行趋势。方法 收集2000年与2010年四川大学华西医院收治的初诊为原发性支气管肺癌并登记为四川地区常住人口的病例,对两组患者的性别、年龄、城乡来源、吸烟史、职业暴露、病理类型等临床资料进行对比分析。结果 收集肺癌病例共2 167例,其中2000年616例,2010年1 551例。肺癌患者男女比由2000年的2.78∶1下降至2010年的2.13∶1(P =0.013)。2000年与2010年肺癌患者发病年龄差异无统计学意义(P =0.302)。地域分布上,十年间大城市及中小城市肺癌患者构成比下降(大城市: 42.1% vs. 32.0%, P PP=0.041;农村: 12.5% vs. 28.2%, P PPP

英文摘要

【Abstract】 Objective To construct the sh-rpS6 lentivirus vector targeting ribosomal protein S6 (rpS6) and explore its effect on proliferation in lung adenocarcinoma A549 cell lines. Methods Sequences targeting the rpS6 gene were selected. The double strand shRNA oligo was ligated to pGCsil-GFP lentivirus vector and transformed into E.coli. The resulting recombinant vector was verified by sequencing. After transfection and lentivirus packing, the viral particles were collected and infected A549 cells. After selection of GFP positive cells by FACS, mRNA and protein expression levels of rpS6 were determined by real time PCR and Western blot. In the following experiment, the proliferation changes of A549 cell lines after the interference by sh-rpS6 was investigated by using CCK-8 kit. Results The sequencing result confirmed that pGCsil-sh-rpS6-GFP vector was successfully developed. Stably transfected A549 cell lines by sh-rpS6 were selected through FACS, with a selection ratio of 86.80%. The silencing effects of sh-rpS6 were determined by real time PCR and Western blot, suggesting that mRNA and protein expression of rpS6 in the targeted cells reduced by (79.72±6.83)% and (83.77±12.13)%, significantly lower than those of control groups. In vitro showed the cell proliferation with sh-rpS6 was significantly slower than that of controls (PrpS6 lentivirus vector could inhibit the expression of rpS6 in A549 cell lines effectively and significantly slow the cell proliferation In vitro

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