Magnetic particle chemiluminescence kit for detecting frazolidone metabolites and application of magnetic particle chemiluminescence kit
A chemiluminescence reagent and furazolidone technology, which is applied to a magnetic particle chemiluminescence kit for detecting furazolidone metabolites and its application field, can solve the problems of poor reagent stability, the influence of reaction time and temperature, and achieves low detection time and fast detection. , the effect of high sensitivity
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Embodiment 1
[0036] Example 1 Preparation of specific components of the kit
[0037] 1. Preparation of luminescent markers
[0038] a) Synthesis of hapten
[0039] The furazolidone metabolite is derivatized to obtain the furazolidone derivative hapten.
[0040] b) Preparation of luminescent markers
[0041] Take 4.5mmol / L ABEI, dissolve it in 4ml distilled water, dissolve 5.0mmol / L N-hydroxysuccinimide in 0.5ml N,N-dimethylformamide, mix the two well and react at room temperature for 3-4h . Take 15 mg of the furazolidone metabolite hapten prepared above, adjust the volume to 1.5 ml with pH 7.4 PBS, then add the above activated ABEI solution, mix well, react overnight at room temperature, and purify it on a G-25 gel column.
[0042] 2. Preparation of fluorescent markers
[0043] a) Preparation of immunogen:
[0044] The furazolidone metabolite derivative hapten and bovine serum albumin are coupled by a diazotization method to obtain an immunogen.
[0045] b) Preparation of monoclonal antibodies to fura...
Embodiment 2
[0057] Example 2 Construction of the kit
[0058] A magnetic particle chemiluminescence detection kit for the detection of furazolidone metabolites was constructed to contain the following components:
[0059] FITC-labeled fluorescent label of furazolidone metabolite monoclonal antibody
[0060] Luminescent label of ABEI-labeled furazolidone metabolite hapten
[0061] Separation reagent of paramagnetic nanobeads coated with goat anti-FITC monoclonal antibody
[0062] Furazolidone metabolite standard solution (0ng / ml, 0.01ng / ml, 0.03ng / ml, 0.09ng / ml, 0.27ng / ml, 0.81ng / ml), the standard dilution is pH7.4, containing 0.05% thimerosal Preservative, 0.1mol / LTRIS buffer. The percentage is the percentage by mass.
[0063] The concentration of the furazolidone metabolite control solution was 0.02ng / ml and 0.5ng / ml respectively, the quality control substance was diluted to pH7.4, containing 0.05% thimerosal preservative, 0.1mol / L TRIS buffer. The percentage is the percentage by mass.
[0064] T...
Embodiment 3
[0065] Example 3 Detection of furazolidone metabolites in actual samples
[0066] 1. Sample pretreatment
[0067] (1) Pre-processing methods for muscle and liver tissue
[0068] Homogenize the sample with a homogenizer; weigh 1.0±0.05g of the homogenized tissue sample (liver sample / meat sample), add 4ml of deionized water, 0.5ml of 1M hydrochloric acid solution and 100μl of derivatization reagent, fully use a shaker Shake for 2min; incubate at 37℃ overnight (about 16h); add 5ml 0.1M dipotassium hydrogen phosphate solution, 0.4ml 1M sodium hydroxide solution and 5ml ethyl acetate respectively, shake vigorously with a shaker for 30s; 3000g above, room temperature (20- 25℃) Centrifuge for 10min; take 2.5ml ethyl acetate phase into 10ml dry glass test tube and blow dry under nitrogen stream in a water bath at 50~60℃; add 1ml n-hexane (or n-heptane), vortex for 30s with a vortexer, Then add 1ml of reconstituted working solution and mix thoroughly with a vortexer for 1min; centrifuge for...
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