Immunofluorescence test strip component for quickly and quantitatively detecting myocardial creatine kinase isozyme, detection card component comprising same and preparation method
A creatine kinase, quantitative detection technology, applied in the field of laboratory medicine, can solve the problems of high missed diagnosis rate, expensive equipment, low positive rate, etc., and achieve the effect of low cost, sufficient response and simple operation
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Embodiment 1
[0057] like figure 1 As shown, a test strip assembly for rapid quantitative detection of myocardial creatine kinase isoenzyme, including a test strip and a platinum porphyrin-labeled specific antibody used in conjunction with the test strip and independently packaged, the test strip includes a substrate 1 , the water-absorbing pad 2, the coating analysis membrane 3 and the sample pad 6 sequentially bonded on the substrate, the coating analysis membrane 3 is provided with a detection line 4 and a quality control line 5, and the specific antibody coated on the detection line 4 is anti- Myocardial creatine kinase isoenzyme monoclonal antibody, the specific antibody coated by quality control line 5 is rabbit IgG antibody; platinum porphyrin-labeled specific antibody is anti-myocardial creatine kinase isoenzyme monoclonal antibody and anti-rabbit IgG antibody.
[0058] Among them, one side of the bottom liner 1 of the test strip is coated with adhesive or double-sided tape, which i...
Embodiment 2
[0099] In step 2, the preparation method of the detection line coating solution is: 20mM pH7.6 Tris buffer solution (TAPS buffer solution), containing 0.8% methanol, 1% sucrose, 0.6% bovine serum albumin, 10M50 antibody 1mg / ml. Preparation of quality control line coating solution: 50mM pH7.6 phosphate buffer (PB buffer), containing 0.7% methanol, 0.5% bovine serum albumin, and 0.5mg / ml rabbit IgG. Preparation of the coating film: debug the BIO-DOT film spraying machine, the film liquid volume is 20ul / 40cm, the machine is scribed, the distance between the detection line and the quality control line is 5mm, the scribed line is fine and uniform, and it is placed in a vacuum drying oven at 25°C-37°C for 1.5 Hours, bagged and sealed for later use.
Embodiment 3
[0101] The preparation method of the present embodiment is basically the same as that of the first embodiment, the difference is that:
[0102] In step 3, the anti-CK-MB monoclonal antibody and anti-rabbit IgG antibody were diluted to 1mg / ml with 0.1M sodium bicarbonate solution respectively, and 5ml of antibody solution was taken respectively, and 40mg of fluorescein platinum porphyrin solution was added respectively, and stirred Mix well, incubate at room temperature for 1.5 hours, and mix every 15 minutes. Finally, use a G25 gel column to separate and purify, collect the labeled fluorescein-labeled antibody, and use a gel containing 0.01%-0.5% polyethylene glycol, 1%-5% bovine serum albumin, 5%-20% glycerol, 0.01% -0.05% surfactant diluted with 0.01M phosphate buffer solution, packaged in a sealed plastic bottle, and stored at 4°C.
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