重庆医科大学学报
重慶醫科大學學報
중경의과대학학보
UNIVERSITATIS SCIENTIAE MEDICINAE CHONGQING
2009年
12期
1617-1621
,共5页
李春蕾%何晓燕%彭琼乐%张政%武卫华%彭惠民
李春蕾%何曉燕%彭瓊樂%張政%武衛華%彭惠民
리춘뢰%하효연%팽경악%장정%무위화%팽혜민
miRNA-451%iNOS基因%肾小球系膜细胞%基因表达
miRNA-451%iNOS基因%腎小毬繫膜細胞%基因錶達
miRNA-451%iNOS기인%신소구계막세포%기인표체
MiRNA-451%iNOS gene%Mesangial cell%Gene expression
目的:探讨miRNA-451对肾小球系膜细胞中诱导型一氧化氮合酶(Inducible nitric oxide synthase,iNOS)基因表达的影响.方法:依据miRBase数据库中mmu-miR-451序列,设计两条寡核苷酸片段,退火处理后克隆至pGenesil-1质粒,构建pGenesil-1-miRNA-451质粒及阴性对照质粒pGenesil-1-control.将pGenesil-l-miRNA-451及pGenesil-1-control质粒分别转染小鼠肾小球系膜细胞,经G418筛选,建立稳定表达pGenesil-1-miRNA-451及pGenesil-1-control的细胞株.采用MTT比色法检测活细胞数并绘制生长曲线;RT-PCR、Western blot及免疫细胞化学检测iNOS基因表达的差异.结果:经测序证实重组质粒构建成功,与未处理的小鼠肾小球系膜细胞和稳定表达pGenesil-1-control的细胞相比,在稳定表达pGenesil-1-miRNA-451的小鼠肾小球系膜细胞中,细胞增殖受到抑制,iNOS基因的蛋白表达明显受到抑制,而iNOS基因的mRNA水平无明显变化.结论:miRNA-451在翻译水平抑制了iNOS基因的表达,并对小鼠肾小球系膜细胞生长具有显著的抑制作用.
目的:探討miRNA-451對腎小毬繫膜細胞中誘導型一氧化氮閤酶(Inducible nitric oxide synthase,iNOS)基因錶達的影響.方法:依據miRBase數據庫中mmu-miR-451序列,設計兩條寡覈苷痠片段,退火處理後剋隆至pGenesil-1質粒,構建pGenesil-1-miRNA-451質粒及陰性對照質粒pGenesil-1-control.將pGenesil-l-miRNA-451及pGenesil-1-control質粒分彆轉染小鼠腎小毬繫膜細胞,經G418篩選,建立穩定錶達pGenesil-1-miRNA-451及pGenesil-1-control的細胞株.採用MTT比色法檢測活細胞數併繪製生長麯線;RT-PCR、Western blot及免疫細胞化學檢測iNOS基因錶達的差異.結果:經測序證實重組質粒構建成功,與未處理的小鼠腎小毬繫膜細胞和穩定錶達pGenesil-1-control的細胞相比,在穩定錶達pGenesil-1-miRNA-451的小鼠腎小毬繫膜細胞中,細胞增殖受到抑製,iNOS基因的蛋白錶達明顯受到抑製,而iNOS基因的mRNA水平無明顯變化.結論:miRNA-451在翻譯水平抑製瞭iNOS基因的錶達,併對小鼠腎小毬繫膜細胞生長具有顯著的抑製作用.
목적:탐토miRNA-451대신소구계막세포중유도형일양화담합매(Inducible nitric oxide synthase,iNOS)기인표체적영향.방법:의거miRBase수거고중mmu-miR-451서렬,설계량조과핵감산편단,퇴화처리후극륭지pGenesil-1질립,구건pGenesil-1-miRNA-451질립급음성대조질립pGenesil-1-control.장pGenesil-l-miRNA-451급pGenesil-1-control질립분별전염소서신소구계막세포,경G418사선,건립은정표체pGenesil-1-miRNA-451급pGenesil-1-control적세포주.채용MTT비색법검측활세포수병회제생장곡선;RT-PCR、Western blot급면역세포화학검측iNOS기인표체적차이.결과:경측서증실중조질립구건성공,여미처리적소서신소구계막세포화은정표체pGenesil-1-control적세포상비,재은정표체pGenesil-1-miRNA-451적소서신소구계막세포중,세포증식수도억제,iNOS기인적단백표체명현수도억제,이iNOS기인적mRNA수평무명현변화.결론:miRNA-451재번역수평억제료iNOS기인적표체,병대소서신소구계막세포생장구유현저적억제작용.
Objective:To elucidate the effect of miRNA-451 on the expression of inducible nitric oxide synthase(iNOS)gene in the mesangial cells of mice.Methods:Two template DNA sequences were designed based on mmu-miR-451 sequence in miRBase database.The mmu-miR-451 expression plasmid and a control plasmid,named pGenesil-1-miRNA-451 and pGeneil-1-control respectively,were generated by the cloning of annealed oligonueleotides into pGenesil-1,then transfected into mesangial cells,which were stably selected by G418 to establish mesangial cell lines stablely expressing pGenesil-1-miRNA-451 and pGenesil-1-control.The living cells were counted by MTT assay and cell growth curves were drew to analyze the cell proliferation.The iNOS mRNA level was assessed by RT-PCR.The expression of iNOS protein was determined by Western blot and immunocytochemistry.Results:The recombinant vectors were verified by sequencing.The cell growth curves indicated the proliferation of cells transfected with pGenesil-1-miRNA-451 were inhibited significantly,compared with that of cells transfected with pGenesil-control and cells without treatments.RT-PCR analysis showed the levels of iNOS mRNA were almost unchanged in the cells with or without treatments.Western blot and immunocytochemistry demonstrated a significant decrease of iNOS protein level in the cells transfected with pGenesil-1-miRNA-451,but not in the cells transfected with pGenesil-1-control,when compared with mesangial cells.Conclusion:miRNA-451 repressed the expression of iNOS gene translafionly,and significantly inhibited cell growth.