Magnetic particle chemiluminescence kit for detecting trenbolone, and applications thereof
A chemiluminescence reagent and kit technology, applied in chemiluminescence/bioluminescence, analysis by chemical reaction of materials, measurement devices, etc., can solve the problems of poor reagent stability, reaction time and temperature effects, etc. The effect of low time, fast detection and high sensitivity
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Embodiment 1
[0035] The preparation of the concrete component of embodiment one kit
[0036] 1) Synthesis of Trenbolone Hapten
[0037] Synthesize trenbolone hapten from trenbolone by succinic anhydride method.
[0038] 2) Preparation of artificial antigen
[0039] The trenbolone hapten and bovine serum albumin were coupled to the immunogen by the carbodiimide method.
[0040] 3) Preparation of monoclonal antibodies
[0041] Animal immunization: Immunize Balb / c mice with the immunogen at a dose of 100 μg / mouse to produce antiserum.
[0042] Cell fusion and cloning: Splenocytes from immunized Balb / c mice were fused with SP2 / 0 myeloma cells at a ratio of 9:1 to obtain hybridoma cell lines of monoclonal antibodies.
[0043] Cell cryopreservation and recovery: the hybridoma cells were made into 1×10 cryopreservation medium 9 cells / ml for long-term storage in liquid nitrogen. When recovering, take out the cryopreservation tube, put it into a 37°C water bath to thaw quickly, remove the cry...
Embodiment 2
[0054] The formation of embodiment two kits
[0055] The magnetic particle chemiluminescence kit for detection of trenbolone was assembled to contain the following components:
[0056] Fluorescent marker of FITC-labeled trenbolone monoclonal antibody
[0057] Luminescent marker of ABEI-labeled trenbolone hapten
[0058] Separation reagent of paramagnetic nanobeads coated with goat anti-FITC monoclonal antibody
[0059] Trenbolone standard solution (0ng / ml, 0.01ng / ml, 0.03ng / ml, 0.1ng / ml, 0.5ng / ml, 1.0ng / ml), the standard diluent is pH7.4, 0.03%NaN 3 , 0.1mol / LPBS buffer. The percentage content is a mass percentage content.
[0060] The concentrations of Trenbolone quality control solution are 0.02ng / ml and 0.8ng / ml respectively, and the quality control dilution solution is pH7.4, 0.03% NaN 3 , 0.1mol / LPBS buffer. The percentage content is a mass percentage content.
[0061] Concentrated lotion is PH7.2, 0.2-0.4% Tween-20, 0.2-0.4% NaN 3 , 0.1-0.2mol / L PBS buffer soluti...
Embodiment 3
[0062] The detection of trenbolone in the actual sample of embodiment three
[0063] 1. Sample pretreatment
[0064] (1) Feed, tissue (chicken / liver, pork / liver, shrimp, fish, etc.) pretreatment method
[0065] Use a homogenizer to homogenize tissue and feed samples; weigh 2.0±0.05g of homogenate into a 50ml polystyrene centrifuge tube, add 10ml of acetonitrile-0.1M sodium hydroxide solution, shake with an oscillator for 10min, over 3000g, and store at room temperature ( 20-25°C) and centrifuge for 10min; pipette 0.5ml supernatant into a 50ml polystyrene centrifuge tube, add 0.5ml 0.1M sodium hydroxide solution, add 5ml chloroform after shaking, vortex for 2min with a vortex instrument, Above 3000g, centrifuge at room temperature (20-25°C) for 10min. (If the sample is emulsified, put it in a water bath at 70°C for 2-4 minutes, and centrifuge again until the lower layer is clear); remove the upper layer, take 1ml of the lower layer of clear organic phase into a 10ml clean gla...
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