Patent ID: 11959912
Assignee: WUHAN NEWCANDO BIOTECHNOLOGY CO., LTD.
Field: Measurement (Instruments)
Classification: CPC G | IPC G

Claim 0:
1. A preparation method of a fluorescence immunochromatographic detection card comprising a treatment liquid (A), a treatment liquid (B), and a detection card, in which the treatment liquid (A) contains a first antibody that is coupled with a carboxylated fluorescent microsphere formed by embedding fluorescent molecules and the first antibody targets an antigen to be tested; the treatment liquid (B) contains a second antibody that is coupled with biotin and the second antibody targets the antigen to be tested; the first antibody is an antibody 15C4, and the second antibody is an antibody 13G12; the detection card comprises a detection line area and a quality control line area, a streptavidin detection T line is fixed in the detection area, and an antibody quality control C line is immobilized in the quality control line area;
wherein the preparation method comprises the following steps:
(1) preparing the treatment liquid (A);
(1.1) adding a first quantity of 1-ethyl-3-(3-dimethylamino-propyl) carbodiimide hydrochloride and a second quantity of N-hydroxy-succinimide into a third quantity of carboxylated fluorescent microspheres thereby obtaining a first mixture solution and performing activation thereby obtaining a fourth quantity of activated carboxylated fluorescent microspheres, after the activation, centrifuging the first mixture solution, and then collecting a precipitate of the first mixture solution in a phosphate buffer, and dispersing the precipitate of the first mixture solution in the phosphate buffer to acquire a dispersion liquid of the activated carboxylated fluorescent microspheres;
(1.2) adding a fifth quantity of the first antibody into the dispersion liquid of the activated carboxylated fluorescent microspheres prepared in the step (1.1) thereby obtaining a second mixture solution for a coupling reaction, and then centrifuging the second mixture solution, and collecting a sediment of the second mixture to acquire a sixth quantity of the first antibodies coupled with the activated carboxylated fluorescent microspheres;
(1.3) adding a seventh quantity of bull serum albumin to the sixth quantity of the first antibodies coupled with the activated carboxylated fluorescent microspheres prepared in (1.2) to block a surface of the activated carboxylated fluorescent microspheres thereby obtaining a third mixture solution, and then centrifuging the third mixture solution and collecting a sediment of the third mixture solution, adding an antibody storage buffer into the third mixture solution to acquire the treatment liquid (A);
(2) preparing the treatment liquid (B):
adding an eighth quantity of the second antibody into a biotin solution thereby obtaining a fourth mixture solution for the coupling reaction, and then diluting the fourth mixture solution and dialyzing the fourth mixture solution to eliminate excess unreacted biotin, collecting samples of the fourth mixture solution to acquire the treatment liquid (B);
(3) drawing the line on the detection card;
immobilizing a streptavidin solution onto the test area to form the T line, and immobilizing an antibody solution onto the quality control line to form the C line.