中华手外科杂志
中華手外科雜誌
중화수외과잡지
CHINESE JOURNAL OF HAND SURGERY
2014年
5期
391-395
,共5页
李波%弓贺炜%李文斌%李永平%冯勇%贾英伟%田江华%李刚%梁炳生
李波%弓賀煒%李文斌%李永平%馮勇%賈英偉%田江華%李剛%樑炳生
리파%궁하위%리문빈%리영평%풍용%가영위%전강화%리강%량병생
细胞分化%细胞增殖%慢病毒载体%L6成肌细胞%微小RNA-133a%MEF2A
細胞分化%細胞增殖%慢病毒載體%L6成肌細胞%微小RNA-133a%MEF2A
세포분화%세포증식%만병독재체%L6성기세포%미소RNA-133a%MEF2A
Cell differentiation%Cell proliferation%Lentiviral vector%L6 myoblasts%Micro RNA-133a%MEF2A
目的 构建微小RNA-133a重组慢病毒载体,观察其转染后对L6成肌细胞增殖、分化及转录因子MEF2A的影响.方法 构建表达含微小RNA-133a基因的重组慢病毒载体,转染L6成肌细胞,以实时定量PCR(Taqman探针法)对微小RNA-133a基因表达水平进行检测;细胞计数试剂盒(CCK-8)试验评价微小RNA-133a过表达后对L6成肌细胞增殖的影响;倒置荧光显微镜观察L6成肌细胞增殖、分化的影响;Western blot法检测转录因子MEF2A表达水平的变化.结果 构建的微小RNA-133a重组慢病毒载体经质粒酶切和测序鉴定正确;与对照组比较,转染L6成肌细胞24h后,微小RNA-133a基因的相对表达量明显增加(P<0.01);L6细胞增殖数量明显增加(P<0.01),对L6成肌细胞的分化有明显抑制作用(P<0.01);MEF2A的表达量逐渐下降(P<0.01).结论 成功构建微小RNA-133a重组慢病毒载体并转染16成肌细胞后可高效表达微小RNA-133a,促进体外成肌细胞的增殖并抑制分化.
目的 構建微小RNA-133a重組慢病毒載體,觀察其轉染後對L6成肌細胞增殖、分化及轉錄因子MEF2A的影響.方法 構建錶達含微小RNA-133a基因的重組慢病毒載體,轉染L6成肌細胞,以實時定量PCR(Taqman探針法)對微小RNA-133a基因錶達水平進行檢測;細胞計數試劑盒(CCK-8)試驗評價微小RNA-133a過錶達後對L6成肌細胞增殖的影響;倒置熒光顯微鏡觀察L6成肌細胞增殖、分化的影響;Western blot法檢測轉錄因子MEF2A錶達水平的變化.結果 構建的微小RNA-133a重組慢病毒載體經質粒酶切和測序鑒定正確;與對照組比較,轉染L6成肌細胞24h後,微小RNA-133a基因的相對錶達量明顯增加(P<0.01);L6細胞增殖數量明顯增加(P<0.01),對L6成肌細胞的分化有明顯抑製作用(P<0.01);MEF2A的錶達量逐漸下降(P<0.01).結論 成功構建微小RNA-133a重組慢病毒載體併轉染16成肌細胞後可高效錶達微小RNA-133a,促進體外成肌細胞的增殖併抑製分化.
목적 구건미소RNA-133a중조만병독재체,관찰기전염후대L6성기세포증식、분화급전록인자MEF2A적영향.방법 구건표체함미소RNA-133a기인적중조만병독재체,전염L6성기세포,이실시정량PCR(Taqman탐침법)대미소RNA-133a기인표체수평진행검측;세포계수시제합(CCK-8)시험평개미소RNA-133a과표체후대L6성기세포증식적영향;도치형광현미경관찰L6성기세포증식、분화적영향;Western blot법검측전록인자MEF2A표체수평적변화.결과 구건적미소RNA-133a중조만병독재체경질립매절화측서감정정학;여대조조비교,전염L6성기세포24h후,미소RNA-133a기인적상대표체량명현증가(P<0.01);L6세포증식수량명현증가(P<0.01),대L6성기세포적분화유명현억제작용(P<0.01);MEF2A적표체량축점하강(P<0.01).결론 성공구건미소RNA-133a중조만병독재체병전염16성기세포후가고효표체미소RNA-133a,촉진체외성기세포적증식병억제분화.
Objective To construct recombinant lentiviral vector of micro RNA-133a and observe the proliferation,differentiation and expression of transcription factor MEF2A of L6 myoblasts transfected with the vector system.Methods Recombinant lentiviral vector containing micro RNA-133a gene was constructed and transfected into L6 myoblasts.The expression of micro RNA-133a gene was detected by real-time PCR (Taqman probe).The effect of micro RNA-133a overexpression on L6 myoblast proliferation was quantified using cell counting kit (CCK-8).Its effect on cell differentiation was detected by inverted fluorescence microscope.Western blot assay was used to detect the expression level of transcription factor MEF2A in these cells.Results The successful construction of micro RNA-133a recombinant lentiviral vector was confirmed by plasmid enzyme digestion and DNA sequencing.Compared with the control group,relative expression of micro RNA-133a gene in L6 myoblasts was significantly increased (P < 0.01) 24h after the vector transfection.L6 cell proliferation was increased significantly (P < 0.01),while its differentiation was effectively inhibited.The expression level of MEF2A was significantly reduced (P < 0.01).Conclusion Micro RNA-133a recombinant lentiviral vector can successfully transfect L6 myoblasts causing the cells to overexpress micro RNA-133a.This overexpression promotes L6 myoblast proliferation and inhibits its differentiation in an in vitro cell culture system.