Kit for detecting albumen and application thereof
A kit and protein technology, applied in biological testing, measuring devices, material inspection products, etc., can solve the problem that secreted proteins cannot be directly detected
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[0057] In the present invention, the preparation method of the conjugate of the goat anti-mouse IgG and quantum dots comprises the following steps:
[0058] S1. Dissolve the quantum dots in the activation solution, then add Sulfo-NHS and EDC solution in sequence, activate for 3-8 minutes, centrifuge to discard the supernatant, and dissolve the obtained precipitate with the activation solution to obtain an activated quantum dot solution;
[0059] The activation solution is 5mM BS buffer solution with a mass concentration of 0.01% Tween 20 and a pH value of 7.4;
[0060] S2. Mix goat anti-mouse IgG with the activated quantum dot solution obtained in step S1, and react in the dark for 10-16 hours at 4°C, then add BSA with a mass concentration of 8-15%, react at 37°C for 20-40min, and add washing solution, centrifuged to remove the supernatant, the precipitate was dissolved in the washing solution, and the supernatant was removed by centrifugation again, the precipitate was dissol...
Embodiment 1
[0099] 1. Coupling of PAMAM and goat anti-rabbit IgG:
[0100] (1) Chelating the strong positive charge at the amino terminus of PAMAM G5
[0101] Dissolve 60mg of PAMAM in 2ml of DMSO, stir at room temperature until dissolved, add 0.246g of succinic anhydride, shake the shaker at 180 for 4 hours, and operate in the dark throughout the process to obtain the modified PAMAM solution.
[0102] (2) Prepare a 3500MWCO dialysis bag, boil it with 1 L of 2% sodium bicarbonate, 1 mmol / LEDTA.Na2 solution for 10 minutes, and then filter and wash it with double distilled water.
[0103] (3) Transfer the modified PAMAM solution to a 3500MWCO dialysis bag for 24 hours of dialysis, then freeze-dry the dialysate, weigh it (0.057g), and record the freeze-dried product as cPAMAM.
[0104] (4) Configure MES buffer, take 4.26g MES and dissolve in 200ml water;
[0105] Prepare MES solution of NHS, take 0.023g NHS and dissolve in 4ml of MES buffer;
[0106] Prepare the MES solution of EDC, take ...
Embodiment 2
[0154] Kit for the detection of cytokine Hsp27
[0155] Description: MCF-7 breast cancer cells are used as positive cells (corresponding results are as follows Figure 9-A , Figure 9-A It is the flow diagram of L02 cells, the left picture is a scatter diagram and the right picture is a unimodal diagram).
[0156] Take L02 human normal liver cells as negative cells (the corresponding results are as follows Figure 9-B , Figure 9-B It is the flow diagram of MCF-7 cells, the left picture is a scatter diagram and the right picture is a single peak diagram).
[0157] Antigen Hsp27 was captured with mouse anti-Hsp27 and rabbit anti-Hsp27 as primary antibodies.
[0158] Add PAMAM-conjugated goat anti-rabbit IgG, incubate at 37°C for 30 minutes, and divide the incubated product into two;
[0159] Take one part of the above-mentioned bisected product and add quantum dot-coupled goat anti-mouse IgG, incubate at 37°C for 30 minutes, and the other part will not be treated. It is us...
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