Detection method of nitrate and nitrite in blood, urine and tissue
A technology of nitrite and detection method, which is applied to the content of nitrate and nitrite in urine and tissue, and the field of accurate determination of human or animal blood. It can solve the problems of difficult to meet the detection requirements, interference with experimental results, and low content. , to achieve the effect of improving detection sensitivity, eliminating mutual interference, and eliminating interference
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Embodiment 1
[0025] The invention is used to detect the content of nitrate and nitrite in human urine.
[0026] 1. Production of nitrate and nitrite working curve: take 0.20, 0.4, 0.6, 0.80, 1.00mL NO respectively 3 - (200μg / mL) and NO 2 - (20μg / mL) The standard stock solution is diluted to 5mL in five 10mL centrifuge tubes, and the concentrations are respectively 8.0, 16.0, 24.0, 32.0, 40.0μg / mL and 0.8, 1.6, 2.4, 3.2, 4.0μg / mL. Add 150μL GriessA reagent and mix well. Add 150μL GriessB reagent after 1min, mix well, leave it for 5min, inject 10μL under the mobile phase conditions described in Table 1, and measure at 220nm and 510nm wavelength respectively; regression equation, correlation coefficient, relative standard deviation, recovery rate, etc. See Table 2.
[0027] Table 2 Linear equation of nitrate and nitrite
[0028]
[0029]
[0030] 2. Sample processing and measurement results
[0031] Take 10mL urine in a 10mL centrifuge tube, add 1.0g activated carbon, mix well, centrifuge at 4000r / ...
Embodiment 2
[0033] The invention is used to detect the content of nitrate and nitrite in rabbit urine.
[0034] 1. According to Example 1, make the working curve of nitrate and nitrite.
[0035] 2. Sample processing and measurement results
[0036] Take 2.0mL urine in a 10mL centrifuge tube, add 0.2g sepiolite, mix well, centrifuge at 5000r / min for 15min, filter paper to remove sepiolite. Take 1.0 mL of decolorized urine in a 10 mL centrifuge tube, add 30 μL GriessA reagent, and mix well. Add 30μL GriessB reagent after 1min, mix well, leave it for 5min, use Table 1 as the mobile phase conditions, inject 10μL, measure at 220nm and 510nm wavelengths respectively, and substitute the peak areas obtained into the working curve of Table 2 to obtain The nitrate content was 11.43μg / mL, and nitrite was not detected.
Embodiment 3
[0038] The invention is used to detect the content of nitrate and nitrite in human blood.
[0039] 1. According to Example 1, make the working curve of nitrate and nitrite.
[0040] 2. Sample processing and measurement results
[0041] Take 5mL of fresh blood and centrifuge at 5000r / min for 25min. Take the supernatant in a centrifuge tube, add 0.1 mL of 10% (w / v) sodium hydroxide solution and 1 mL of 5% (w / v) zinc sulfate solution, mix well, centrifuge at 10000r / min for 10 minutes, and take the supernatant 1.0 Add 50μL GriesssA reagent to 10mL centrifuge tube and mix well. After 1 min, add 50μL GriesssB reagent, mix well, leave it for 5min, use Table 1 as the mobile phase conditions, inject 10μL, measure at 220nm and 510nm wavelengths respectively, and substitute the peak areas obtained into the working curve of Table 2 to obtain The nitrate content is 9.53μg / mL, and the nitrite content is 0.08μg / mL.
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