Test paper strip for rapidly detecting brucellosis antibody
A Brucella, detection test paper technology, applied in the preparation of Brucella outer membrane protein bp26 genetically engineered antigen, Brucella antibody rapid detection test strip field, can solve indeterminate, especially medical history, contact History, occupation, eating habits, living areas and endemic areas, lack of simple, fast, specific and sensitive detection methods, insufficient knowledge of brucellosis, etc., to achieve the effect of saving manpower and material resources, easy promotion, storage and transportation
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Embodiment 1
[0033] Embodiment 1: the preparation of Brucella outer membrane protein bp26 genetic engineering antigen
[0034] (1) Obtaining the target gene
[0035] According to the sequence of the target gene fragment (GenBank accession number is AY166769) and the characteristics of the pGEX-4T-1 (Pharmacia) expression vector, primers containing restriction enzymes EcoR1 and Xho1 restriction sites at both ends were designed:
[0036] 5'gaattcatgaacactcgtgct3'
[0037] 5'gcctcgagttacttgatttcaa3'
[0038] Then, the target gene fragment bp26 was amplified from the Brucella genome. The amplification conditions were: denaturation at 95°C for 5 minutes; 1 minute at 95°C, 1 minute at 49.8°C, and 1 minute at 70°C for 35 cycles; finally, extension at 70°C for 10 minutes.
[0039] (2) Cloning of the target gene and screening of positive recombinants
[0040] After electrophoresis, the PCR amplified product was recovered by gel cutting, ligated with the PMD-18T cloning vector overnight at 16°C, ...
Embodiment 2
[0049] Example 2: Preparation of polyclonal antibody against outer membrane protein bp26
[0050] (1) Animal immunity:
[0051] Select 1-2kg New Zealand white rabbits, and inject bp26 protein subcutaneously in multiple points on the back, and the immunization dose is 1mg / kg. A total of 4 times of immunization.
[0052] (2) Immunological titer detection:
[0053] ELISA plate coated with bp26 protein, 4 μg per well. The titer of immune serum was detected by indirect ELISA method. When the serum titer reaches 1:20000 or more, serum can be collected.
[0054] (3) Antibody purification and verification:
[0055] Purification by conventional octanoic acid method. The purity was tested by non-denaturing PAGE electrophoresis, showing a protein band. The activity is tested by ELISA, and the titer is greater than 1:20000.
Embodiment 3
[0056] Embodiment 3: the development of Brucella antibody detection kit
[0057] (1) Preparation of colloidal gold-antigen conjugate:
[0058] It was determined by experiments that when bp26 protein was used as the gold-labeled antigen, the optimal binding pH value was 8.0, and the protein ratio was 46 μg / ml colloidal gold. After the labeled colloidal gold is treated with a stabilizer (0.5% BSA, pH8.0, 0.01M Tris buffer), take the colloidal gold-antigen conjugate solution in an amount of 65 μl per square centimeter, evenly adsorb it on the glass fiber, and freeze-dry it. , and stored in a dry environment.
[0059] (2) Coating antigen on nitrocellulose membrane:
[0060] The Brucella outer membrane protein bp26 was diluted to 3.5 ± 0.1 mg / ml with 0.01 M PBS. Dilute goat anti-mouse IgG polyclonal antibody to 2±0.1mg / ml with 0.01M PBS. Spray the two on the nitrocellulose membrane at a speed of 1 μl / cm with a film spraying machine to form a test line and a control line, respec...
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