Application of methyl-β-cyclodextrin in preparation of medicine for preventing and treating silkworm cells infected by bmnpv
A technology of cyclodextrin and silkworm, applied in the direction of antiviral agent, etc., can solve the problems of non-patent and literature reports, etc.
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Embodiment 1
[0024] 1. Construction of BmNPV carrying egfp reporter gene
[0025] The hsp70-egfp fragment was cloned into the BamHI (Takara) and NotI (Takara) sites of pFastBacDual (Invitrogen), the donor plasmid pFastBacDual-hsp70-egfp was constructed, and BmBac-egfp was obtained by transposition (see schematic diagram figure 1 ), after BmBac-egfpDNA was transfected into BmN (bombyx mori ovary cells) cells, green fluorescent expression could be observed under a fluorescent microscope. The cell supernatant was used to infect BmN cells, and the virus was harvested 72 hours after infection, and the virus titer was determined by the terminal dilution method, and the virus was stored in a refrigerator at 4°C in the dark.
[0026] 2. Inoculation of cells and preparation of stock solution of MβCD (Sigma)
[0027] (1) Inoculate about 10 cells in a 35mm cell culture dish (Corning) respectively. 5 Add 2 mL of 10% FBS TC100 insect cell culture medium to each cell dish of BmN cells.
[0028] (2) C...
Embodiment 2
[0037] When the final concentration of MβCD is 4mM, the prevention and treatment of BmNPV infection carrying egfp reporter gene:
[0038] (1) Take 10 of each inoculation 5 3 culture dishes of cells, remove the old culture medium, add 105.2 μL MβCD storage solution and 894.8 μL 10% FBS TC100 medium to the 3 cell culture dishes respectively, so that the final concentration of MβCD in the culture dish is 4 mM, 27 °C After culturing for 30 minutes, remove the medium containing MβCD, wash twice with serum-free TC100 medium, and shake gently for 3 minutes each time.
[0039] (2) After washing the cells, remove the washing solution, add BmBac-egfp virus with MOI=10, and infect the cells at 27° C. for 1 hour.
[0040] (3) After 1 hour, wash twice with serum-free TC100 medium, shake gently for 3 minutes each time, remove the washing solution, add 2 mL of 10% FBS TC100 medium, and incubate at 27°C for 6 hours.
[0041] (4) After 6 hours, place 3 dishes in a fluorescent confocal micros...
Embodiment 3
[0043] When the final concentration of MβCD is 6mM, the prevention and treatment of BmNPV infection carrying egfp reporter gene:
[0044] (1) Take 10 of each inoculation 5 3 culture dishes of cells, remove the old medium, add 157.8 μL MβCD storage solution and 842.2 μL 10% FBS TC100 medium to the 3 cell culture dishes respectively, so that the final concentration of MβCD in the culture dish is 6 mM, 27 °C Cultivate for 30 minutes, remove the medium containing MβCD, wash twice with serum-free TC100 medium, shake gently, each time for 3 minutes.
[0045] (2) After washing the cells, remove the washing solution, add BmBac-egfp virus with MOI=10, and infect the cells at 27° C. for 1 hour.
[0046] (3) After 1 hour of infection, wash twice with serum-free TC100 medium, shake gently for 3 minutes each time, remove the washing solution, add 2 mL of 10% FBS TC100 medium, and incubate at 27°C for 6 hours.
[0047] (4) After 6 hours, place 3 dishes in a fluorescent confocal microscope...
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