Purification Packaging, Titer and Detection of c-myc Retrovirus Expression Vector
zeng Rong,Li fin,Zhou Sheng(The First Military Medical University, Guangzhou, 510515)
Abstract:In order to obtain high transfective ability of retroviral constructure, WizardTM DNA purification system was applied to three kinds of antisense c-myc retroviral expression vectors which used to transfect PA317 package cells with lipofectine, then viral titers were assayed and external gene integration were examined by neo gene PCR amplification. The results indicated that the purified DNA accorded with the demands of eukaryonic cell transfection, however, the viral titers were influenced by the growth of target cells and the number of PA317 sampling in the meanwhile. Neo gene PCR amplification was also indicated a sensitive, economical and reliable test for gene integration.
Keywords:c-myc; retrovirus vector参考文献:
[1]Housma DE. A new retrovirus packaging cell for gene transfer constructed from amplified long terminal repeat-free chimeric proviral genes. J virol, 1992, 66: 3725
[2]Vile R, Russell SJ. Gene transfer technologies for the gene therapy of cancer. Gene Therapy, 1994, 1: 88
[3]Miller AD, Buttimore C. Redesign of retrovirus packaging cell lines to avoid recombination leading to helper virus production. Mol Cell biol, 1986, 6(8): 2895
[4]Kazunori A, Teruhiko Y, Takashi S, et al. Liposome-mediated in vivo gene transfer of antisense k-ras construct inhibits pancreatic tumor dissemination in the murine peritoneal cavity. Cancer res, 1995, 55: 3810
[5]郭宁,李秀森,毛宁,等。K562细胞导入IL-2基因后的细胞凋亡,实验血液学杂志,1995, 3(4): 364
