中国癌症防治杂志
中國癌癥防治雜誌
중국암증방치잡지
CHINESE JOURNAL OF ONCOLOGY PREVENTION AND TREATMENT
2015年
4期
244-249,250
,共7页
张智%朱广志%彭涛%赵国良%徐静
張智%硃廣誌%彭濤%趙國良%徐靜
장지%주엄지%팽도%조국량%서정
肝肿瘤%组织蛋白酶S%过表达%慢病毒%增殖%迁移
肝腫瘤%組織蛋白酶S%過錶達%慢病毒%增殖%遷移
간종류%조직단백매S%과표체%만병독%증식%천이
Liver neoplasm%Cathepsin S%Overexpression%Lentivirus infections%Proliferation%Migration
目的:建立慢病毒介导过表达组织蛋白酶S (cathepsin S,Cat S)基因的肝癌细胞株,观察Cat S基因对肝癌MHCC97H细胞增殖和迁移的影响。方法利用Age I和EcoR I双酶切获得目的基因片段,构建靶向过表达Cat S基因的慢病毒载体pLVX-EGFP-3FLAG-Puro,通过人胚肾上皮293T细胞进行慢病毒制备并感染肝癌MHCC97H细胞。使用嘌呤霉素加压筛选,建立稳定过表达Cat S基因的肝癌细胞株。通过RT-PCR、Western blot、MTT、Transwell和划痕实验研究稳定过表达Cat S基因对肝癌MHCC97H细胞增殖和迁移的影响。结果成功包装靶向过表达Cat S基因慢病毒载体并感染肝癌MHCC97H细胞。慢病毒感染后,与空载对照细胞Mock-MHCC97H相比,慢病毒Cat S-MHCC97H细胞Cat S mRNA、Cat S蛋白及MMP-2蛋白表达量明显升高(P<0.05),细胞增殖、迁移、侵袭能力亦明显增强(P<0.05)。结论慢病毒介导的Cat S基因过表达可能通过上调MMP-2蛋白表达促进肝癌MHCC97H细胞增殖、转移,Cat S基因可能是治疗肝癌的一个潜在靶点,这为阐明肝癌增殖和转移的分子生物学机制及提高肝癌基因治疗提供了新的实验依据。
目的:建立慢病毒介導過錶達組織蛋白酶S (cathepsin S,Cat S)基因的肝癌細胞株,觀察Cat S基因對肝癌MHCC97H細胞增殖和遷移的影響。方法利用Age I和EcoR I雙酶切穫得目的基因片段,構建靶嚮過錶達Cat S基因的慢病毒載體pLVX-EGFP-3FLAG-Puro,通過人胚腎上皮293T細胞進行慢病毒製備併感染肝癌MHCC97H細胞。使用嘌呤黴素加壓篩選,建立穩定過錶達Cat S基因的肝癌細胞株。通過RT-PCR、Western blot、MTT、Transwell和劃痕實驗研究穩定過錶達Cat S基因對肝癌MHCC97H細胞增殖和遷移的影響。結果成功包裝靶嚮過錶達Cat S基因慢病毒載體併感染肝癌MHCC97H細胞。慢病毒感染後,與空載對照細胞Mock-MHCC97H相比,慢病毒Cat S-MHCC97H細胞Cat S mRNA、Cat S蛋白及MMP-2蛋白錶達量明顯升高(P<0.05),細胞增殖、遷移、侵襲能力亦明顯增彊(P<0.05)。結論慢病毒介導的Cat S基因過錶達可能通過上調MMP-2蛋白錶達促進肝癌MHCC97H細胞增殖、轉移,Cat S基因可能是治療肝癌的一箇潛在靶點,這為闡明肝癌增殖和轉移的分子生物學機製及提高肝癌基因治療提供瞭新的實驗依據。
목적:건립만병독개도과표체조직단백매S (cathepsin S,Cat S)기인적간암세포주,관찰Cat S기인대간암MHCC97H세포증식화천이적영향。방법이용Age I화EcoR I쌍매절획득목적기인편단,구건파향과표체Cat S기인적만병독재체pLVX-EGFP-3FLAG-Puro,통과인배신상피293T세포진행만병독제비병감염간암MHCC97H세포。사용표령매소가압사선,건립은정과표체Cat S기인적간암세포주。통과RT-PCR、Western blot、MTT、Transwell화화흔실험연구은정과표체Cat S기인대간암MHCC97H세포증식화천이적영향。결과성공포장파향과표체Cat S기인만병독재체병감염간암MHCC97H세포。만병독감염후,여공재대조세포Mock-MHCC97H상비,만병독Cat S-MHCC97H세포Cat S mRNA、Cat S단백급MMP-2단백표체량명현승고(P<0.05),세포증식、천이、침습능력역명현증강(P<0.05)。결론만병독개도적Cat S기인과표체가능통과상조MMP-2단백표체촉진간암MHCC97H세포증식、전이,Cat S기인가능시치료간암적일개잠재파점,저위천명간암증식화전이적분자생물학궤제급제고간암기인치료제공료신적실험의거。
Objective To construct a lentivirus expression vector to drive stable Cat S overexpression in the hepatocellular carcinoma (HCC)cell line MHCC97H,and to investigate the effects of overexpression on cell proliferation and migration. Methods The Cat S gene was inserted into the lentiviral expression vector pLVX-EGFP-3FLAG-Puro using Age I and EcoR I restriction enzymes and transfected into 293T cells to generate recombinant lentivirus. This virus was used to infect MHCC97H cells,and positive cells were selected using puromycin. Real-time quantitative PCR,Western blots,MTT assay,the transwell migration assay and the wound healing migration assay were used to assess the effects of Cat S overexpression on proliferation and migration of MHCC97H cells. Results A lentiviral vector containing the Cat S gene was constructed,and an MHCC97H cell line stably overexpressing Cat S was established. Cat S overexpression was associated with significantly shorter cell doubling time,as well as significantly greater invasion and migration abilities. Conclusions Lentivirus-mediated Cat S overexpression can increase MHCC97H proliferationand migration,opening the door to future studies of molecular mechanisms of liver cancer invasion and metastasis.
