Immunofluorescence reagent strip for determining urinary nuclear matrix protein as well as preparation method and application thereof
A nuclear matrix protein and immunofluorescence technology, applied in the field of quantitative detection of concentration, can solve problems such as low specificity, and achieve the effect of simple and convenient operation and reduced operation time.
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Embodiment 1
[0031] Example 1: Preparation of specific monoclonal antibody against nuclear matrix protein (NMP22)
[0032] 1. Animal immunity:
[0033]Female Balb / c mice aged 6-8 weeks were selected as immunization objects. Before the initial immunization, blood was collected from the tail vein of each mouse, and 200 μl of the emulsified immunogen (antigen plus complete adjuvant) was injected intraperitoneally during the initial immunization; after the initial immunization On the 14th day and the 28th day, the second and third immunizations (antigen plus incomplete adjuvant) were carried out in the same way. On the 5th day after the third immunization, blood was collected from the orbit of each mouse to collect serum to evaluate the antibody effect. On the seventh day after the third immunization, booster immunization was carried out, and 100 μl of immunogen was injected into the tail vein. On the third day after the booster immunization, spleen lymphocytes and SP2 / 0 (mixing ratio of 5:1) ...
Embodiment 2
[0041] An immunofluorescence reagent strip for measuring urinary nuclear matrix protein, characterized in that: in the immunofluorescence reagent strip, water-absorbing pads, chromatographic membranes, binding pads, and sample pads are arranged in sequence; the sample pad corresponds to the sample adding area, and the binding pad Corresponding to the binding area; the chromatographic membrane corresponds to the detection area; the chromatographic membrane is equipped with a detection line T line and a quality control line C line; the detection line T line is coated with NMP22 monoclonal antibody N-C2; the quality control line C line Goat anti-mouse IgG is coated on the top; antibody complex Cy3-N-C1 labeled with fluorescent substances is laid on the binding pad.
[0042] T-line and C-line diluent formula: 0.01M PBS, 5% sucrose, 1% BSA; binding pad treatment solution formula: 0.1MTris-HCl, 0.1% Tween-20, 0.5% PVA, 5% sucrose, 1% BSA; Cy3-N-C1 diluent formula: 0.01MPBS, 0.5% PVA...
Embodiment 3
[0054] Example 3: Standard Curve for Determination of Urinary Nuclear Matrix Protein Immunofluorescence Reagent Strip
[0055] The NMP22 antigen solution can be diluted with antigen diluent to a final concentration of 0ng / mL, 4ng / mL, 8ng / mL, 16ng / mL, 32ng / mL, 64ng / mL serial standard solution.
[0056] Antigen diluent is 0.05mol / L phosphate buffer containing BSA and sucrose, pH=7.4, containing 20gBSA, 50g sucrose, 8g NaCl, 0.2g KCl, 0.24g KH per liter 2 PO 4 , 1.44 g Na 2 HPO 4 of aqueous solution.
[0057] According to the detection steps of the urine nuclear matrix protein NMP22 immunofluorescence reagent strip assay method, the fluorescence detection intensity of the NMP22 series standard products was obtained. According to the fluorescence intensity value and concentration of the standard as the coordinate axis, select a suitable mathematical model to establish a standard curve, the standard curve is as follows figure 2 As shown, the correlation coefficient r=0.9982 w...
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