Seneca valley virus structural protein epitope polypeptide and application thereof
A technology of structural proteins and antigenic epitopes, applied in the direction of viral peptides, viruses, viruses/bacteriophages, etc., can solve problems such as difficulties in clinical differential diagnosis, and achieve the effects of less antigen consumption, strong specificity, and improved efficiency
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Embodiment 1
[0046] Example 1, Preparation of Seneca Valley Virus Structural Protein Antibody ELISA Kit Coating Antigen
[0047] In this experiment, bioinformatics methods were used to accurately analyze the main epitopes of the Seneca Valley virus structural proteins VP1, VP2, and VP3, and suitable peptides were screened out. Four peptides were synthesized with an automatic peptide synthesizer, and the sequences were respectively As shown in Sequence 1, Sequence 2, Sequence 3 and Sequence 4 in the sequence listing, a newer and more complete coating antigen with a purity of about 80% is made, which can cover the main neutralizing antigenic epitope of Seneca Valley virus, and improve Antibody positive detection rate. The polypeptide synthesis method can be a conventional method. The following method is used in the present invention to synthesize the four polypeptides of the present invention as the coating agent of the kit of the present invention.
[0048] The coated antigen of the presen...
Embodiment 2
[0077] Example 2, Preparation of Seneca Valley Virus Structural Protein Antibody ELISA Kit
[0078] Seneca Valley Virus Structural Protein Antibody ELISA Kit includes:
[0079] (1) 96-well detachable polystyrene enzyme-linked reaction plate coated with Seneca Valley virus antigen; 2×96 wells.
[0080] (2) Positive control serum: pig serum collected after artificial infection with Seneca Valley virus was used as the positive control serum of the kit (1 tube, 1.5ml / tube).
[0081] (3) Negative control serum: specific pathogen-free (SPF) pig serum, used as the negative control serum of the kit (1 tube, 1.5ml / tube).
[0082] (4) Enzyme-labeled secondary antibody: prepared by diluting 1:30000 with horseradish peroxidase-labeled rabbit anti-pig IgG (purchased from sigma company, product number A5670) as the stock solution, 2 bottles (12ml / bottle).
[0083] (5) Sample diluent: 0.01M phosphate buffer containing 0.5% (g / 100ml) casein, pH 7.4, 1 bottle (24ml / bottle).
[0084] (6) Sub...
Embodiment 3
[0090] Example 3, Sensitivity Test of Seneca Valley Virus Structural Protein Antibody ELISA Kit
[0091] 1. How to use the Seneca Valley Virus Structural Protein Antibody ELISA Kit
[0092] 1. Equilibration: Take the kit out of the refrigerated environment, and put it at room temperature for 30 minutes for later use; mix the liquid reagents before use.
[0093] 2. Dosing: dilute the 20-fold concentrated washing solution with distilled water or deionized water 20 times to obtain the washing buffer;
[0094] 3. Setting: 2 negative control wells and 2 positive control wells, and the rest are sample wells to be tested.
[0095] 4. Pre-dilution of the specimen to be tested: use the sample diluent to dilute the serum of the sample to be tested, the negative control serum, and the positive control serum at a ratio of 1:20.
[0096] 5. Adding samples: Add 100 μl of diluted samples to be tested in each well according to the preset setting. The time span of adding samples should be as ...
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