Quick biological sample detection method
A detection method and technology for biological samples, applied in the field of medical rapid diagnosis and detection, can solve the problems of difficulty in the accuracy and precision of detection results, residues, insufficient response, etc., to achieve improved accuracy and precision, complete information, The effect of low background signal
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Embodiment 1
[0017] In order to describe the content of the present invention more clearly, the following takes C-reactive protein (CRP) as an example for further description. Double-antibody sandwich method, 1000nm carboxy-modified magnetic beads, europium-chelated fluorescent particles, and anti-CRP antibodies 1 and 2. Antibody 1 and antibody 2 used mouse anti-human MC01 antibody and MC02 antibody of Hangzhou Qitai Biotechnology, respectively.
[0018] The binding of CRP antibody 1 to magnetic beads can be prepared by the following method:
[0019] (1) Washing and dispersion of magnetic beads: wash with 50mmol / l MES buffer and disperse in MES buffer.
[0020] (2) Activation of magnetic beads: Weigh activator EDC and NHS and dissolve in (1) magnetic bead solution, the concentration of activator is 100mg / ml, react for 10 minutes. Wash and disperse with MES buffer, and the concentration of activated magnetic beads is 10mg / ml.
[0021] (3) Connection between magnetic beads and antibody: t...
Embodiment 2
[0031] In order to describe the content of the present invention more clearly, the N-terminal pro-brain natriuretic peptide (NT-proBNP) detection item is taken as an example for further description below. Using double-antibody sandwich method, 200nm carboxy-modified magnetic beads, europium-chelated fluorescent particles (excitation light is about 300nm, emission light is about 600nm), antibody 1 uses NT‐proBNP produced by Hytest company with batch number: 13 / 01-8NT2 Antibody; Antibody 2 using the batch number produced by Hytest Company: 13 / 02-NT1-G12 anti-antibody.
[0032] The combination of NT-proBNP antibody 1 and magnetic beads is the same as Example 1:
[0033] The combination of NT-proBNP antibody 2 and fluorescent particles is the same as in Example 1.
[0034] The composition of the sample treatment solution in the NT‐proBNP in vitro diagnostic kit: Tris‐HCl50mmol / l), Casein (0.5%), Tween‐20 (1%), magnetic beads combined with NT‐proBNP antibody 1, and NT‐proBNP antib...
Embodiment 3
[0037] In order to describe the content of the present invention more clearly, the procalcitonin (PCT) detection item is taken as an example for further description below. Double-antibody sandwich method, 200nm carboxy-modified magnetic beads, AMCA fluorescent particles from Thermo Fisher (excitation light is about 340nm, emission light is about 440nm), antibodies are mouse anti-human MJG03 antibody and MJG05 from Hangzhou Qitai Biotechnology Antibody.
[0038] The combination of PCT antibody 1 and magnetic beads is the same as Example 1:
[0039] The combination of PCT antibody 2 and fluorescent particles is the same as in Example 1.
[0040]The composition of the sample treatment solution in the PCT in vitro diagnostic kit: Tris‐HCl 50mmol / l), Casein (0.5%), Tween‐20 (1%), magnetic beads combined with PCT antibody 1, and fluorescent particles combined with PCT antibody 2.
[0041] The analysis process is as follows, add 90ul sample to 10ul sample treatment solution, then m...
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