Composition for enzyme linked immunosorbent assay kit, anti-nuclear antibody spectrum detection kit and preparation method thereof
An enzyme-linked immunosorbent reagent and composition technology, which is applied in measurement devices, biological material analysis, instruments, etc., can solve the problems of high cost, complicated operation of protein chips, low stability, etc., and achieve the effect of optimal stability.
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Embodiment 1
[0038] Embodiment 1: Preparation of antinuclear antibody spectrum detection kit of the present invention
[0039] 1. Coating of nuclear component antigens and related proteins
[0040] The PC, NC, S1, S2, S3, S4, S5, and EC points in the protein chip array are coated with 2ug / ml, 0.01ug / ml, 0.1ug / ml, 0.5ug / ml, 2ug / ml, 4ug respectively / ml, 8ug / ml, 2ug / ml of human IgG, the dilution buffer is CB buffer at pH9.6 (which contains 2.5% PEG4000, 5% trehalose, 0.05% Proclin300, and 15% glycerol) .
[0041] SC dots are coated with 2ug / ml goat anti-human IgG antibody, and the dilution buffer is CB buffer at pH 9.6.
[0042] Loc dots are coated with 2ug / ml human IgG, and the dilution buffer is CB buffer at pH 9.6.
[0043] The 7 antigens of dsDNA, Sm, U1RNP, Scl-70, Jo-1, histone, and nucleosome were respectively treated with 0.01M PBS buffer of pH7.4-PH7.6 (containing 0.5% PVP, 5% Trehalose, 0.05% Proclin300, 0.02% 2-hydroxy-β-cyclodextrin) were diluted, and the final concentrations...
Embodiment 2
[0068] Embodiment 2: Stability detection of the kit of the present invention
[0069] Control kit: prepared according to the method of Example 1, the difference is that the blocking solution is a conventional PBS buffer solution containing 3% BSA and 0.05% Proclin300, pH7.4; the enzyme label diluent uses the enzyme in the prior art CN105021811A Standard diluent: 0.46% tris, 5% goat serum, 0.8% NaCl, 0.1% Tween 20, 0.04% EDTA, 0.5% sodium paraben, 0.1% Proclin300, the balance is deionized water.
[0070] Test kit: embodiment 1 kit;
[0071] Detection method: place the two kits at room temperature (18-28°C) and low temperature (2-8°C) for a period of time, then use the same serum to detect according to the detection method in Example 1, and count the signal value of the instrument. The results are shown in Table 2-5.
[0072] 1. The stability data of the kit in Example 1 at low temperature
[0073] Table 2
[0074]
[0075]
[0076]
[0077] As can be seen from Table...
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