Time-resolved fluoroimmunoassay kit for detecting fumonisins B1 and detection method thereof
A technology of time-resolved fluorescence and fumonisins, which is used in analytical materials, fluorescence/phosphorescence, material excitation analysis, etc., can solve the problems of expensive equipment, complicated operation, low sensitivity, etc., and achieves simple structure, convenient use and sensitivity. high effect
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Embodiment 1
[0019] Example 1 Preparation of kit and detection of corn samples
[0020] The reagents provided in the kit are enough for 96 measurements, and the materials in the box are as follows:
[0021] (1). 1 x 96-well plate (8 strips x 12 wells, which can be split into single wells) coated with FB1-BSA.
[0022] (2). 6×FB1 standard solution, 1.0mL / bottle, the concentration of the standard solution is: 0, 1.0, 10, 100, 500, 1000ng / mL.
[0023] (3). 1× FB1 monoclonal antibody freeze-dried product, dissolved in 0.5mL distilled water.
[0024] (4).1×Eu 3+ - Lyophilized goat anti-mouse antibody, dissolved in 0.5mL distilled water.
[0025] (5). 1× enhancement solution: 15mL.
[0026] (6). 1×washing solution: 30mL, dilute with distilled water 1:25 when used.
[0027] (7). 1× buffer solution: 30 mL.
[0028] Reagents that should be prepared by the laboratory
[0029] Methanol.
[0030] 70% Methanol Solution: Prepare 70% methanol solution by mixing 30mL distilled or deionized water a...
Embodiment 2
[0044] The reagents provided in the kit are enough for 48 measurements, and the coated plate in the box is: 1×48 well plate (4 strips×12 wells, which can be split into single wells) coated with FB1-BSA. The remaining reagents provided by the kit are the same as in Example 1 and are used to detect wheat samples. The specific detection steps are as follows:
[0045] The wheat sample is firstly processed: crush the wheat sample to 20 mesh, take 5 grams of the crushed wheat sample and put it in a test tube, add 25 mL of extract (methanol:water=7:3). Stopper and vibrate for 3 minutes, filter, and use Xinhua No. 1 paper as the filter paper. Take 1mL of the filtrate and dilute it with 9mL of distilled or deionized water for later use.
[0046] Take the FB1-BSA strip, add 50 μL of FB1 standard or processed samples to their respective microwells, add 50 μL of FB1 monoclonal antibody diluted 1:20 in buffer, shake at 25°C for 1 hour, wash with washing solution 3 times, Add 1:20 dilute...
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