Method, reagent and kit for quantitative determination of NGAL content in human serum
A technology for lipocalin and neutrophils, which is applied in biological tests, measuring devices, material inspection products, etc., can solve the problems of high price, unsuitable for routine inspection, waste of resources, etc., and achieves easy operation and fully automated analysis. Effect
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Embodiment 1
[0023] Configure the following reagent I and reagent II of the present invention according to the following ingredients and ratios:
[0024] Reagent I:
[0025] Phosphate buffer 30mmol / L
[0026] Polyethylene glycol 8000 30mmol / L
[0027] Reagent II:
[0028] Mouse anti-human NGAL monoclonal antibody latex particles 50mL / mol
[0029] Antibody stabilizer 0.05g / mL
[0030] Mix 240 μl reagent I and 3 μl serum sample in a sample tube, incubate at 37°C for 5 minutes, use Hitachi 7060 automatic biochemical analyzer, measure the absorbance A1 of the sample relative to the blank tube at a wavelength of 546 nm, and then add Mix 60 μl of reagent II, incubate at 37°C for 5 minutes, and measure the absorbance A2 of the sample relative to the blank tube. Calculate the ΔA sample according to the following formula (1). Use the same method and conditions to measure the absorbance value of the standard solution, and calculate the △A standard. Then calculate the neutrophil gelatinase-ass...
Embodiment 2
[0035] Configure the following reagent I and reagent II of the present invention according to the following ingredients and ratios:
[0036] Reagent I:
[0037] Phosphate buffer 150mmol / L
[0038] Polyethylene glycol 8000 150mmol / L
[0039] Reagent II:
[0040] Mouse anti-human NGAL monoclonal antibody latex particles 500mL / mol
[0041] Antibody stabilizer 0.5g / mL
[0042] Mix 240 μl reagent I and 3 μl serum sample in the sample tube, incubate at 37°C for 5 minutes, use the Olympus 400 automatic biochemical analyzer, measure the absorbance A1 of the sample relative to the blank tube at a wavelength of 546 nm, and then Add 60 μl of reagent II to the sample, mix well, incubate at 37°C for 5 minutes, and measure the absorbance A2 of the sample relative to the blank tube. Calculate the ΔA sample according to the following formula (1). Use the same method and conditions to measure the absorbance value of the standard solution, and calculate the △A standard. Then calculate th...
Embodiment 3
[0047] Configure the following reagent I and reagent II of the present invention according to the following ingredients and ratios:
[0048] Reagent I:
[0049] Phosphate buffer 100mmol / L
[0050] Polyethylene glycol 8000 50mmol / L
[0051] Reagent II:
[0052] Mouse anti-human NGAL monoclonal antibody latex particles 300mL / mol
[0053] Antibody stabilizer 0.1g / mL
[0054] Mix 240 μl reagent I and 3 μl serum sample in the sample tube, incubate at 37°C for 5 minutes, use Beckman LX20 automatic biochemical analyzer, measure the absorbance A1 of the sample relative to the blank tube at a wavelength of 546 nm, and then add to the sample Add 60 μl of reagent II, mix well, incubate at 37°C for 5 minutes, and measure the absorbance A2 of the sample relative to the blank tube. Calculate the ΔA sample according to the following formula (1). Use the same method and conditions to measure the absorbance value of the standard solution, and calculate the △A standard. Then calculate th...
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