Schistosomiasis electrochemistry sensing quick determination kit, detection method and preparation method of kit
A technology for rapid determination of schistosomiasis, applied in electrochemical variables of materials, measuring devices, scientific instruments, etc., can solve the problems of early diagnosis of the disease, low sensitivity, and high missed detection rate, and achieves low production cost and crossover. The effect of low reactivity and few reagents
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Embodiment 1
[0025] Example 1 Electrochemical detection of schistosomiasis antibodies using printed carbon electrodes as sensing elements
[0026] Printed carbon electrode surface treatment: The printed carbon electrode is scanned by cyclic voltammetry in PB buffer to activate the electrode, the voltage range is -0.3V~0.6V, the scan rate is 0.5V / s, scan for 10 cycles, and then rinse with ultrapure water , blow dry with nitrogen.
[0027] Sensing interface construction: drop 10ul of an aqueous solution containing 200mM EDC and 50mM NHS on the electrode surface, and react at room temperature for 15min to activate the carboxyl group. Add 10ul of the single SEA antigen and the mixed SjE16 and SEA antigens in different proportions to the surface of the electrode respectively, react at room temperature for 2 hours, rinse the electrode with PBST, and dry it with nitrogen gas. Add 50 ul of 1% BSA dropwise to the surface of the electrode to seal at room temperature for 1 hour, then rinse the elect...
Embodiment 2
[0031] The preparation method of embodiment 2 schistosome electrochemical sensing rapid assay kit
[0032] 1. Preparation of electrochemical sensing array: Rinse the multi-channel printed carbon paste electrode with ultrapure water, add 50ul10mM phosphate buffer (PB) dropwise to cover the three electrodes, and perform cyclic voltammetry on a multi-channel electrochemical detector To scan, rinse the electrodes with ultrapure water. Then drop 10ul carboxyl activation solution containing 200mM carbodiimide (EDC) and 50mM N-hydroxysuccinimide (NHS) on the surface of the working electrode, react at room temperature for 15 minutes, rinse the electrode with ultrapure water, and then On the surface of the working electrode, drop 5ul containing 50mg / L Schistosoma japonicum recombinant antigen SjE16 (provided by the Chinese Center for Disease Control and Prevention of Parasitic Diseases) and 6mg / L of Schistosoma japonicum soluble egg antigen SEA (provided by the Chinese Center for Disea...
Embodiment 3
[0039] The detection method of embodiment 3 schistosome antibody
[0040] 1. Sample dilution:
[0041] Qualitative detection: Dilute the serum to be tested 1:100 with the sample diluent, for example, add 1 μl of serum to 99 μl of diluent, mix thoroughly, and do not need to dilute the negative and positive reference substances.
[0042] Semi-quantitative detection: Dilute the serum to be tested at 1:100 with the sample diluent, and then serially dilute to 3200 times (the dilution factor can be appropriately increased or decreased according to the antibody concentration), and the negative and positive controls do not need to be diluted.
[0043] 2. Sample addition reaction:
[0044] 2.1 Add 10ul of diluted sample serum to each working electrode, and test 2 wells in parallel for each sample. At the same time, set 2 wells for negative, positive and blank controls. Take 10ul of negative and positive control substances and drop them on the surface of the working electrode respectiv...
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