中华实验外科杂志
中華實驗外科雜誌
중화실험외과잡지
CHINESE JOURNAL OF EXPERIMENTAL SURGERY
2014年
11期
2402-2404
,共3页
李志%焦鑫艳%杨岩%徐莲花%张向文%金锦花%李文哲
李誌%焦鑫豔%楊巖%徐蓮花%張嚮文%金錦花%李文哲
리지%초흠염%양암%서연화%장향문%금금화%리문철
小干扰RNA%核心岩藻糖转移酶Fut8%70Z/3-Fut8-RNAi%细胞信号传导
小榦擾RNA%覈心巖藻糖轉移酶Fut8%70Z/3-Fut8-RNAi%細胞信號傳導
소간우RNA%핵심암조당전이매Fut8%70Z/3-Fut8-RNAi%세포신호전도
Small interference RNA%Core fucosyltransferase Fut8%70Z/3-Fut8-RNAi%Cell signal transduction
目的 观察阻抑核心岩藻糖基化修饰对前B细胞信号传导的调节作用.方法 利用逆转录病毒包装技术建立核心岩藻糖转移酶Fut8基因沉默前B细胞株(70Z/3-Fut8-RNAi细胞).用实时定量聚合酶链反应(Real-time PCR)及Western blot检测Fur8 mRNA、蛋白表达和细胞内信号分子的酪氨酸磷酸化水平.结果 成功构建重组pSINsi-hU6-Fut8 siRNA质粒,逆转录病毒包装后病毒滴度可达2.1×105 CFU/ ml.Real-time PCR及Western blot检测结果表明70Z/3-Fut8-RNAi细胞的Fut8基因和蛋白表达明显下降,蛋白表达水平下调70% ~ 80%,mRNA水平下调70% ~80%,以及pre-BCR介导的细胞信号传导,即CD79a及BTK磷酸化显著下降.结论 成功构建70Z/3-Fut8-RNAi细胞株,Fut8修饰的核心岩藻糖基化可能在早期B细胞的细胞信号传导过程中发挥重要的调节作用.
目的 觀察阻抑覈心巖藻糖基化脩飾對前B細胞信號傳導的調節作用.方法 利用逆轉錄病毒包裝技術建立覈心巖藻糖轉移酶Fut8基因沉默前B細胞株(70Z/3-Fut8-RNAi細胞).用實時定量聚閤酶鏈反應(Real-time PCR)及Western blot檢測Fur8 mRNA、蛋白錶達和細胞內信號分子的酪氨痠燐痠化水平.結果 成功構建重組pSINsi-hU6-Fut8 siRNA質粒,逆轉錄病毒包裝後病毒滴度可達2.1×105 CFU/ ml.Real-time PCR及Western blot檢測結果錶明70Z/3-Fut8-RNAi細胞的Fut8基因和蛋白錶達明顯下降,蛋白錶達水平下調70% ~ 80%,mRNA水平下調70% ~80%,以及pre-BCR介導的細胞信號傳導,即CD79a及BTK燐痠化顯著下降.結論 成功構建70Z/3-Fut8-RNAi細胞株,Fut8脩飾的覈心巖藻糖基化可能在早期B細胞的細胞信號傳導過程中髮揮重要的調節作用.
목적 관찰조억핵심암조당기화수식대전B세포신호전도적조절작용.방법 이용역전록병독포장기술건립핵심암조당전이매Fut8기인침묵전B세포주(70Z/3-Fut8-RNAi세포).용실시정량취합매련반응(Real-time PCR)급Western blot검측Fur8 mRNA、단백표체화세포내신호분자적락안산린산화수평.결과 성공구건중조pSINsi-hU6-Fut8 siRNA질립,역전록병독포장후병독적도가체2.1×105 CFU/ ml.Real-time PCR급Western blot검측결과표명70Z/3-Fut8-RNAi세포적Fut8기인화단백표체명현하강,단백표체수평하조70% ~ 80%,mRNA수평하조70% ~80%,이급pre-BCR개도적세포신호전도,즉CD79a급BTK린산화현저하강.결론 성공구건70Z/3-Fut8-RNAi세포주,Fut8수식적핵심암조당기화가능재조기B세포적세포신호전도과정중발휘중요적조절작용.
Objective To investigate the function of core fucosyltransferase Fut8 in the intracellular signal transduction in mice pre-B cells.Methods Using recombinant DNA techniques,complementary 82 bp oligonucleotides designed with hairpin loop for Fut8 siRNA were annealed,and then inserted into the retrovirus expression vector pSINsi-hU6 with BamH Ⅰ and Cla Ⅰ sites.The recombinant retroviral vector pSINsi-hU6-Fut8 siRNA was packaged with 293T cells and the generated recombinant retrovirus infected mice pre B cell line (70Z/3 cells).The expressions of Fut8 mRNA,protein and enzyme activity were detected by Real-time polymerase chain reaction (Real-time PCR),Western blotting and high performance liquid chromatography (HPLC).The phosphorylation of cell signal molecules were detected by Western blotting.Results The restriction enzyme analysis with BamH Ⅰand Cla Ⅰshowed that the recombinant retroviral vector pSINsi-hU6-Fut8 small interference RNA siRNAwas constructed correctly.The titer of generated recombinant retrovirus was up to 2.1 × 105 CFU/ml.The Fut8 mRNA,protein and enzyme activity were significantly down-regulated in Fut8-KD-70Z/3 cells.The pre-BCR-mediated tyrosine-phosphorylation of CD79a and activation of BTK were suppressed in Fut8-KD-70Z/3 cells.Conclusion The Fut8-KD-70Z/3 cells transfected with the pSINsi-hU6-Fut8 siRNA plasmid were established successfully.Core fucosylation mediates the intracellular signaling via pre-BCR in pre-B cells.
