Rabies virus diagnostic reagent kit
A diagnostic kit, rabies virus technology, applied in biological testing, material testing products, measuring devices, etc., can solve the problems of decreased detection sensitivity and difficult purification of the whole virus.
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Embodiment 1
[0021] A rabies virus diagnostic kit, comprising:
[0022] 1) ELISA plate;
[0023] 2) Coating solution: pH 9.4, 50 mmol / L carbonate buffer (CB);
[0024] 3) Enzyme marker: horseradish peroxidase-labeled mouse anti-rabbit enzyme-labeled antibody;
[0025] 4) Chromogenic agent: TMB (3.3.5.5 tetramethylbenzidine) chromogenic solution;
[0026] 5) Washing solution: pH 7.2 PBST phosphate buffer solution;
[0027] 6) Substrate solution: PH5.0 jujube citric acid phosphate
[0028] 7) Stop solution: 2M H 2 SO 4 ;
[0029] 8) Negative control: negative serum of rabies virus standard dog;
[0030] 9) Positive control: Positive serum of rabies virus standard dog.
Embodiment 2
[0032] A kind of rabies virus diagnostic kit, the process of this diagnostic kit working optimal condition optimization is as follows:
[0033] Judgment basis for the best reaction conditions: process the data of each reaction, calculate the P / N value of the reaction, take the largest P / N value, and the P value close to 1 as the judgment basis for the best reaction conditions of indirect ELISA P / N value Calculation method: P / N = (average OD450 nm value of positive control wells - average OD450 nm value of blank control wells) / (average OD450 nm value of negative control wells - average OD450 nm value of blank control wells), characterized by: the ultraviolet light wave is 450nm.
[0034] 1. Selection of the best antigen coating solution
[0035] 50 mmol / L pH 9.4 carbonate buffer (CB), 20 mmol / L pH 8.5 Tris-Hcl (TB), pH 7.2 PBS buffer, pH 7.2 PBST buffer, distilled water (W), normal saline ( S) As a coating solution, dilute the rabies virus protein at a fixed concentration (8...
Embodiment 3
[0048] Embodiment 3: the effect experiment of rabies virus diagnostic kit
[0049] 1. Determination of critical value
[0050]40 samples of normal chicken serum (SPF) were randomly selected, tested according to the above-mentioned indirect ELISA method, and the average OD value (x) and standard deviation SD of the 40 samples of serum were calculated. + 3SD, it can be judged as positive at the 99.9% level. According to statistics, the average value of 40 negative sera is 0.210, and the standard deviation is 0.024, then the critical value = 0.210+3×0.024=0.282. It can be seen that when the OD450 value of the sample is ≥0.281, it can be tested with 99% confidence When the OD450 value of the sample is less than 0.281, it can be judged as negative with 99% confidence.
[0051] 2. Specificity test
[0052] The canine distemper, canine parvovirus, and canine parainfluenza virus positive sera were tested according to the above ELISA operating procedures, and the rabies virus positi...
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