摘要
目的 建立hIL-2基因修饰的人肝细胞株并探讨对其生物学活性的影响。 方法应用重组逆转录病毒载体pLNCIL-2,将hIL-2基因导入人肝细胞系L-02,观察其形态及克隆形成率的变化,检测细胞培养上清中hIL-2的含量,以及进行转染细胞基因组DNA NeoR基因片段的PCR扩增。结果L-02/IL-2细胞的增殖速度和克隆形成率低于L-02/Neo细胞和L-02细胞。L-02/IL-2细胞的培养液中hIL-2的含量达32 000 pg/106cells·d,并可持续表达10 wk以上。从L-02/IL-2细胞和L-02/Neo细胞基因组DNA中,均扩增到NeoR基因片段(790 bp)。结论应用重组逆转录病毒载体成功地建立了L-02/IL-2细胞株,为进一步进行肝细胞移植动物实验奠定了基础。
Aim To establish human hepatocyte line L-02 transfected with pLNCIL-2 and explore the effect of this vector on the biological feasures of the cells. Methods Human interleukin-2 gene was transferred into the L-02 cells by the aid of recombinant retroviral vector pLNCIL-2, then change of morphology and colonogeneicity of the transferred cells were observed. At the same time, the level of hIL-2 secretion in cultural supernatant was detected and NeoR gene were amplified by PCR. Results Proliferation and colonogeneicity of the L-02 /IL-2 cells were lower than those of L-02/Neo and L-02 cells. hIL-2 level secreted reached to 32 000pg/106cells per day and the secretion could gone on for more than ten weeks. In addition, NeoR gene segment was obtained by PCR from both L-02/IL-2 and L-02/Neo cell's genomic DNA. ConclusionhIL-2 gene has been integrated successfully into genomic DNA of human hepatocytes L-02. This result lay the foundation for further research.
出处
《细胞与分子免疫学杂志》
CAS
CSCD
北大核心
2002年第2期146-148,共3页
Chinese Journal of Cellular and Molecular Immunology
基金
福建省科技厅基金资助
No.98A056
