Hybridoma cell strain for secreting anti 1-amino-hydantoin monoclonal antibody and application of hybridoma cell strain
A hybridoma cell line and monoclonal antibody technology, applied in the biological field, can solve the problems of small batches of antibodies, large differences between batches, and less ascites in mice
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Embodiment 1
[0039] The hybridoma cell line 2G9A3-35H11 was delivered to the China Center for Type Culture Collection (Address: China. Wuhan. Wuhan University) on August 26, 2015. The viability of the cell line was tested on September 10, 2015. The result was survival , deposit number CCTCC No: C2015141.
[0040] The hybridoma cell line uses the conjugate (AHD-CP-BSA) of derivatives of nitrofurantoin metabolites (AHD-CP) and bovine serum albumin (BSA) as an antigen to immunize BALB / c mice, and the mice after immunization The splenocytes of the splenocytes were fused with the rejuvenated SP2 / 0 myeloma cells, cultured in medium without adding antibiotics, and obtained after screening and 6 times of cloning. The specific process is as follows:
[0041] 1. Hapten synthesis
[0042]Weigh 300 mg of p-4-carboxybenzaldehyde (4-Carboxybenzaldehyde, 4-CBA) in 1 mL of distilled water, add dropwise dimethyl sulfoxide (DMF) until 4-CBA is completely dissolved, add 100 mg of nitrofurantoin metabolite ...
Embodiment 2
[0083] F of 2G9A3-35H11 cell line 3 Substitute for the production of monoclonal antibodies, antibodies can be prepared in vivo or in vitro.
[0084] 1. In vivo preparation of AHD monoclonal antibody
[0085] 6-week-old male Balb / c mice were intraperitoneally injected with 0.5 mL of liquid paraffin 2 weeks in advance → take 2×10 6 the F 3 Inject hybridoma cells into the abdominal cavity of mice → 7-12 days later, when the mice are slightly enlarged, inject 1×10 6 hybridoma cells → 2 to 5 days later, when the abdomen of the mouse is enlarged, draw the ascites with a large needle → kill the mouse by guiding the spine, wash the peritoneal cavity with PBS, collect the washing fluid, merge it into the ascites → purify the antibody, each mouse Mice can obtain 5-15 mg of antibody.
[0086] 2. In vitro → preparation of AHD monoclonal antibody
[0087] The 2G9A3-35H11 cell line was inserted into a glass cell bottle, added with 1640 medium (containing 10% fetal bovine serum), at 37°...
Embodiment 3E
[0094] Example 3 ELISA method detects nitrofurantoin metabolites in chicken (application of primary purified antibody)
[0095] (1) Coating: Dilute AHD-CP-OVA to 300ng / mL with carbonate buffer solution of pH=9.6, add 100μL / well into the microwell strip of the microplate, overnight at 4°C, add 200μL to each well after washing the plate 10% skimmed milk powder, sealed at 37°C for 2 hours, washed and dried in the shade for later use.
[0096] (2) Sample pretreatment: Prepare 3 Snow Mountain Ma chicken breast muscle samples, weigh 1±0.05g of homogeneous samples, weigh 12 copies of each sample, and separate them with 1-amino-2-lactoin (AHD) standard solution Do 0, 0.2, 0.5, 1.0 μg / kg addition recovery test, and do 3 parallels for each concentration. Add 4mL deionized water, 0.5mL 1mol / L hydrochloric acid and 100μL 0.01mol / L 2-nitrobenzaldehyde (2-NP) solution to each sample, place in a 56°C water bath for 2h, add 5mL 0.1mol / L K 2 HPO 4 , 0.4mL 1mol / L NaOH and 5mL ethyl acetate, ...
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