Pepsinogen I and II combined detection method and kit thereof
A combined detection technology of pepsinogen, which is applied in the field of combined detection methods and kits of pepsinogen Ⅰ and Ⅱ, can solve the problems of undetectable, high reagent cost, and long time consumption, and achieve the effect of reducing the impact of impurities
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Embodiment 1
[0035] The dual-wavelength fluorescent immunochromatographic combined detection method of pepsinogen I and II of the present invention comprises the following steps:
[0036] 1) Preparation of immunochromatographic test strips: Coat pepsinogen Ⅰ monoclonal antibody, pepsinogen Ⅱ monoclonal antibody and chicken IgY on detection line 1 (T line 1 ), detection line 2 (T line 2) and control line (C line), after drying for 1 to 5 hours, cut with a strip cutter to obtain immunochromatographic test strips with a width of 3 to 5 mm;
[0037] It should be noted that: a) Traditional qualitative immunochromatography uses coated goat anti-mouse antibody as the control line. With the increase of pepsinogen Ⅰ or some anti-mouse antibody blocking agents in the serum, the signal on the control line As it decreases, its signal value cannot be used for calculation, and the accuracy of the signal of the test line has no reference basis. The present invention adopts chicken IgY antibody and goat ...
Embodiment 2
[0048] like Figures 1 to 2As shown, the dual-wavelength fluorescent immunochromatographic detection kit of pepsinogen I of the present invention includes a kit body, a cryopreservation tube, and a diluent bottle, and the kit body includes a plastic liner 1 and is fixed on the plastic liner. The sample pad 2, the immunochromatography test strip 3 and the absorbent paper 6, the immunochromatography test strip is made of nitrocellulose membrane material, the sample pad and the absorbent paper are respectively lapped on both sides of the immunochromatography test strip, and the immunochromatography test strip is The chromatography test strip is provided with detection line 1 (T1) 4, detection line 2 (T2) 11 and control line 5, and the detection line 1, detection line 2 and control line are respectively coated with pepsinogen Ⅰ monoclonal antibody , pepsinogen Ⅱ monoclonal antibody and chicken IgY; freeze-dried probes were stored in the cryopreservation tube, and the lyophilized p...
specific Embodiment
[0052] The present invention also provides a specific embodiment of dual-wavelength fluorescence immunochromatographic detection of pepsinogen I, which includes the following steps in sequence:
[0053] Step 1: Preparation of lyophilized probes
[0054] 1) Mix two fluorescent latex particle solutions with emission wavelengths of 550nm and 700nm respectively according to the volume ratio of 1:1. After mixing evenly, take 500 μl of mixed fluorescent latex particle solution (containing carboxyl groups) and use pH6.0 MES buffer After washing and centrifuging for three times, the precipitate was diluted with pH6.0 MES buffer, mixed with 10 mg EDC, and then activated at room temperature for 30 minutes. After centrifugation, the precipitate was washed three times with pH6.0 MES buffer, and then the precipitate was washed with pH6. Dilute with 0MES buffer, add 125 μg pepsinogen Ⅰ monoclonal antibody, react at room temperature for 3 hours, add BSA to block, continue to react for 30 min...
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