Duck hemorrhagic oophoritis inactivated vaccine production method by using cell line and product thereof
A technology for hemorrhagic oophoritis and inactivated vaccines, which is applied in the field of vaccine preparation, can solve problems such as the establishment of vaccine evaluation models, the failure to find vaccine strains, and restrictions on vaccine development, and achieve good economic benefits and application prospects. Pollution probability is small, the production process is simple and stable
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Embodiment 1
[0031] Example 1 Screening of virus-adapted cell lines
[0032] According to the characteristics of the virus, four cell lines, bovine embryonic kidney cell line (MDBK), hamster kidney cell line (BHK21), pig kidney cell line (PK15), and African green monkey kidney cell line (Vero), were selected for duck hemorrhagic oophoritis virus. Subculture of HB strain and selection of adaptive cell lines for duck hemorrhagic oophoritis virus.
[0033] All four cells were purchased from China Veterinary Drug Administration.
[0034] Duck hemorrhagic oophoritis virus HB strain, the preservation number is CCTCC V201122, was preserved in China Center for Type Culture Collection on July 1, 2011. The virus is an ssRNA virus with an envelope; the virus particles are roughly spherical, with a diameter of 40-60nm; the virus has strong resistance to the external environment, and it can be stored at 4°C for several weeks and stored at -20°C for several months , its infectivity is not affected;...
Embodiment 2
[0042] Example 2 Breeding of Duck Hemorrhagic Ovarian Virus Strain and Establishment of Virus Seed Batches
[0043] 1 Test method
[0044] 1.1 Breeding of strains
[0045]1.1.1 Virus purification: The duck embryo-adapted strain of duck hemorrhagic oophoritis virus HB strain was successively passaged on hamster kidney cell line (BHK21) and African green monkey kidney cell line (Vero) respectively for 3 times, and the cells were taken to subculture the adapted strain It was purified and cultured using 0.1% neutral red plaque purification technology, continuously purified three times, and the potency was determined;
[0046] 1.1.2 Virus inactivation: Take the cytovenom of the purified virus strains, freeze and thaw twice, add 0.1% formaldehyde of the total amount of cytovenom (V / V) to inactivate, and inactivate by shaking at 37°C for 24 hours;
[0047] 1.1.3 Washing and concentration of venom: The inactivated cell venom is concentrated by ultrafiltration through the Millipo...
Embodiment 3
[0061] Example 3 Preparation of Inactivated Vaccine of Duck Hemorrhagic Ovariitis Using Cell Line
[0062] 1 Test material
[0063] Cell line: hamster kidney cells (BHK21);
[0064] Seed virus: duck hemorrhagic oophoritis virus B propagated in embodiment 2 13 batch;
[0065] Cell growth solution: the composition is 90% DMEM solution by volume, 10% newborn bovine serum, and the pH value is 7.2;
[0066] Cell maintenance solution: the composition is 97% by volume DMEM solution, 3% newborn bovine serum, and the pH value is 7.3.
[0067] 2 Test method
[0068] 2.1 Subculture of cells
[0069] Hamster kidney cells (BHK21) were digested with EDTA-trypsin cell dispersion solution, added cell growth medium, continued to culture at 37°C, and waited for the cells to grow into a good monolayer before use;
[0070] 2.2 Virus inoculation and harvest
[0071] Take the BHK21 cell culture flask that has formed a good monolayer, discard the cell growth medium, and inoculate duck hemor...
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