文章摘要
李珂常青△ 徐平高洪波李贞福 (青.表达增强型绿色荧光蛋白标记的hBax 和hHGF 双基因的慢病毒 载体构建[J].,2012,12(18):3473-3477
表达增强型绿色荧光蛋白标记的hBax 和hHGF 双基因的慢病毒 载体构建
Construction of EGFP Labeled Lentiviral Vector CarryinghBax and hHGF Genes
  
DOI:
中文关键词: 慢病毒载体  肝细胞生长因子  冠状动脉旁路移植术  再狭窄
英文关键词: Lentiviral vector  Hepatocyte growth factor  Coronary artery bypass graft  Restenosis
基金项目:山东省自然科学基金(2005zrb104001)
作者单位
李珂常青△ 徐平高洪波李贞福 (青 青岛大学医学院附属医院 
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中文摘要:
      目的:构建绿色荧光蛋白标记的hBax 和hHGF 双基因共表达的重组慢病毒并鉴定。方法:通过重叠PCR 技术构建attB1- K-hBAX/T2A/eGFP/P2A/hHGF-attB2 基因片段,利用gateway technology 构建慢病毒载体质粒pLV.EX2d.null-EF1A>hBAX/T2A/ eGFP/P2A/hHGF 和阴性对照质粒pLV.EX2d.null-EF1A>eGFP 并测序,上述两种质粒分别与辅助质粒共转染293FT 细胞包装病 毒,荧光显微镜检测病毒滴度。结果:经鉴定慢病毒载体质粒构建正确,荧光显微镜检测hBax 和hHGF 共表达慢病毒滴度为 7.8×107 TU/mL,仅表达绿色荧光蛋白的阴性病毒滴度为9×107 TU/mL。结论:表达增强型绿色荧光蛋白标记的hBax 和hHGF 双基因的慢病毒构建成功并获得高滴度的病毒感染液。
英文摘要:
      Objective: To construct and identify lentiviral vector expressing hBax and Hhgf fusion protein labeled with enhanced green fluorescence protein. Methods: The attB1-K-hBAX/T2A/eGFP/P2A/hHGF-attB2 gene fragment was obtained by overlap PCR method. Gateway technology was used to construct the pLV.EX2d.null-EF1A>hBAX/T2A/eGFP/P2A/hHGF plasmid and pLV.EX2d. null-EF1A>eGFP plasmid. After sequencing, the lenti virus was packaged through co-transfecting above-mentioned construct into human embryonic kidney cell line-293FT with helper plasmids. Then the virus titer was examined by fluorescence microscope. Results: The recombinant lentiviral transfer vector plasmids were constructed correctly, the titer of lentiviral-hBAX-eGFP-hHGF was 7.8×107 TU/mL, and the titer of lentiviral-eGFP was 9×107 TU/mL. Conclusions: The lentiviral vector was constructed and high titer of lentivirus particles were obtained successfully.
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