Method for measuring viral titer of Marek's disease (MD) turkey herpesvirus vaccine, live
A technology of turkey herpes virus and chicken Marek's disease, which is applied in the field of determination of immunogen content, can solve problems such as inaccurate measurement results, unsatisfactory protection, failure of chicken immunity, etc., and achieves simple operation and counting, Low cost and easy to adhere to the wall
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Embodiment 1
[0036] Example 1 Preparation of chicken embryo fibroblasts:
[0037] ⑴ Select well-grown 9-day-old Merial SPF chicken embryos, strictly disinfect the surface of the chicken embryos, use tweezers to knock out the eggshell in the air chamber, carefully clamp the chicken embryos with elbow ophthalmic tweezers, take them out and place them in a sterilized plate ;
[0038] (2) Remove the eyes, brain and internal organs of the chicken embryo, and wash the embryo body three times with 0.01M PBS pH7.2 washing solution;
[0039] (3) Add trypsin solution with a mass concentration of 0.25% preheated at 38°C in proportion to 10ml of each embryo body, and digest under magnetic stirring for 10 minutes each time. After each digestion, the cell solution is filtered through 2 layers of gauze to Add 2% of the total volume of trypsin solution to the container of fetal bovine serum in advance; repeat this step 3 to 4 times;
[0040](4) Centrifuge the cell solution at 2500rpm for 10min, disca...
Embodiment 2
[0045] Example 2 Inoculation of chicken Marek's disease turkey herpesvirus into chicken embryo fibroblast monolayers
[0046] ⑴ Dilute the virus: Select a live chicken Marek’s disease turkey herpes virus vaccine sample (product of Ringpu (Baoding) Biopharmaceutical Co., Ltd., available in the market), use cell maintenance solution (volume percentage 98% M-199 Cell nutrient solution, 2% newborn bovine serum, pH value 7.4) for 1×10 4 and 5×10 4 During the dilution process, use a vortex mixer to mix the virus solution at a speed of 300rpm, and the mixing time is 10-20s to ensure that the virus cell solution is completely mixed;
[0047] (2) Virus inoculation: Discard the cell growth solution in the 24-well cell culture plate, add the diluted virus solution into the wells, and connect 2 dilutions to 5 wells respectively;
[0048] (3) After adding the virus solution, put it in a 38°C incubator for adsorption for 1 hour;
[0049] ⑷ After the adsorption is completed, add 1.5ml...
Embodiment 3
[0050] Example 3 Counting of virus plaques and calculation of virus price:
[0051] The plaques were counted on the 4th day after the virus was inserted, and no plaques appeared in the culture wells of the negative control, and the experiment was established. The plaques in the cell wells were counted under a microscope, from left to right, from top to bottom Observe the plaques in each cell well carefully (some plaques may be fused together, and the germinal centers of the plaques need to be distinguished), according to the number of plaques in each culture well, the volume of the virus solution to be inoculated and the dilution factor Calculate the poisonous price of the virus liquid to be tested.
[0052] Poison Price = The arithmetic mean of each hole plaque at the optimum dilution factor × the optimum dilution factor
[0053] Volume of inoculated virus solution per well
[0054] Note: The optimal dilution factor is the dilution factor in the r...
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