Transgene method of reverse transcription of transfection primitive spermatogonium abduction in virion
A retrovirus, spermatogonial stem cell technology, applied in other methods of inserting foreign genetic materials, genetic engineering, plant genetic improvement, etc., to achieve the effect of simple operation and low investment cost
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Embodiment 1
[0016] Taking LacZ (beta-galactosidase) as the target gene, it was cloned into the downstream of the 5' long terminal repeat (5'-LTR) promoter of the recombinant retroviral vector plasmid pLXSN, and constructed into a packaging vector. The packaging cells PA317 were transfected, and after screening and proliferation, a toxin-producing cell line was obtained, and the supernatant of the cells was collected to concentrate the virus by ultracentrifugation. Dissolve the concentrated virus in phosphate buffer solution (PBS, pH7.2) containing 0.05% (w / v) trypan blue, 0.008g / L Polybrene, operate under a stereoscopic mirror, and inject it for 13-17 days In the seminiferous tubules of young mice. Mice were injected for mating 40 days postoperatively. Take offspring mouse tissues for DNA integration detection (polymerase chain reaction (PCR) uses primers from the nucleic acid sequence of the target gene, and a single nucleotide is catalyzed by a heat-resistant DNA polymerase to elongate...
Embodiment 2
[0019] Taking tPA (tissue plasminogen activator) as the target gene, it was cloned into the 5-LTR of the recombinant retroviral vector pLXSN and downstream of the CMV promoter of pLNCX, and then constructed into a packaging vector, which was transfected into PA317 cells. After screening and proliferation, a toxin-producing cell line is obtained, and the supernatant of the cells is collected to concentrate the virus by ultracentrifugation. Dissolve the concentrated virus in PBS (pH7.2) containing 0.05% (w / v) trypan blue, 0.008g / L Polybrene, operate under a stereoscopic mirror, and inject it into 14-16 day old mice. Inside the seminiferous tubule. Mice were injected for mating 40 days after surgery. The offspring mouse tail tissue was used for DNA integration detection (PCR, Southern hybridization), embryonic fibroblast culture was used for expression detection (RT-PCR), and passage test was carried out. result:
[0020] The toxin-producing cell line transfected with the reco...
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