[Objective]The aim was to explore technical system of making single transgenic positive cells become colony cells by amplification culture. [Method] Fetal fibroblasts and mammary gland epithelial cells of single goat ...[Objective]The aim was to explore technical system of making single transgenic positive cells become colony cells by amplification culture. [Method] Fetal fibroblasts and mammary gland epithelial cells of single goat fetus of pBLM-C1 which specifically expressed human lactoferrin were cloned. Single cell colony of single transfection cell was prepared with 3 concentrations of 0%,50% and 100% conditioned culture media. Transfection cell and non-transfection cell were carried out amplification culture by con-culture,neo gene was as screened gene,genome DNA of transfection cell was detected by PCR method. Chromosome karyotype analysis of single colony cell was tested. [Result] Compared with non-conditioned culture medium,100% conditioned culture medium could greatly increase survived rate of single colony cells (FF: 53.33% vs. 10.00%;MGE: 33.33% vs. 6.67%). Compared with control,con-culture of transfection cell and non-transfection cell could greatly increase rate of transfection cell single colony after amplification culture (FF: 53.33% vs. 10.00%;MGE: 33.33% vs. 6.67%),confluence time of amplification culture was significantly decreased (20-30 d). The result of PCR showed that the colony cell obtained by above method contained hLF target gene. The result of karyotype analysis showed that most cloned cell chromosomes were normal. [Conclusion] The study provides a reliable method for separating transgenic cell,inserting and diagnosing ideal vector,and can save expense and time for transgenic animal production.展开更多
基金Supported by Doctoral Start Fund of Henan University of Science and Technology
文摘[Objective]The aim was to explore technical system of making single transgenic positive cells become colony cells by amplification culture. [Method] Fetal fibroblasts and mammary gland epithelial cells of single goat fetus of pBLM-C1 which specifically expressed human lactoferrin were cloned. Single cell colony of single transfection cell was prepared with 3 concentrations of 0%,50% and 100% conditioned culture media. Transfection cell and non-transfection cell were carried out amplification culture by con-culture,neo gene was as screened gene,genome DNA of transfection cell was detected by PCR method. Chromosome karyotype analysis of single colony cell was tested. [Result] Compared with non-conditioned culture medium,100% conditioned culture medium could greatly increase survived rate of single colony cells (FF: 53.33% vs. 10.00%;MGE: 33.33% vs. 6.67%). Compared with control,con-culture of transfection cell and non-transfection cell could greatly increase rate of transfection cell single colony after amplification culture (FF: 53.33% vs. 10.00%;MGE: 33.33% vs. 6.67%),confluence time of amplification culture was significantly decreased (20-30 d). The result of PCR showed that the colony cell obtained by above method contained hLF target gene. The result of karyotype analysis showed that most cloned cell chromosomes were normal. [Conclusion] The study provides a reliable method for separating transgenic cell,inserting and diagnosing ideal vector,and can save expense and time for transgenic animal production.
