Liquichip for parallel detection of colorectal cancer protein marker, preparation and application thereof
A technology of protein labeling and parallel detection, which is applied in the field of immunology technology and clinical detection, can solve the problem that only one can be detected at a time, which is inconvenient for clinical diagnosis, and achieve the effect of saving detection cost and improving sensitivity and specificity
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Embodiment 1
[0026] Example 1: Coupling of capture antibodies to known numbered microspheres
[0027]1. Select No. 26, 36, 46, 56, 66, 76, and 86 carboxyl microspheres (Luminex Company) respectively, and oscillate the microsphere suspension with a vortex shaker for 20 seconds to mix the microspheres evenly.
[0028] 2. Take about 2×10 carboxyl microspheres of each number above. 3 Transfer each to a centrifuge tube and centrifuge at ≥8000×g for 2 min to precipitate carboxylated microspheres.
[0029] 3. Remove the supernatant and add 100μl dH 2 O, use a vortex shaker to resuspend the microspheres for 20 seconds, centrifuge at ≥8000×g for 2 minutes, and precipitate the carboxylated microspheres.
[0030] 4. Remove the supernatant, add 80 μl, 100 mM, pH=6.2 sodium dihydrogen phosphate salt solution, and resuspend the washed carboxy microspheres with a vortex shaker for 20 seconds.
[0031] 5. Add 10μl, 50mg / ml Sulfo-NHS (with dH 2 O dilution), oscillate gently with a vortex shaker.
[00...
Embodiment 2
[0043] Example 2: Conjugation of detection antibody to biotin
[0044] 1. Dissolve activated biotin (Sigma company) in dimethyl sulfoxide at a concentration of 1 mg / ml.
[0045] 2. The purified detection antibodies to be coupled (respectively: MAb mouse anti-IgGlclone #M111146(10-c10), Mab clone M8073021(10-c04), clone #CA72-4M, MAb-c004-10 mouse anti-IgG1, clone 242 IgG, MAb mouse anti-IgG1 clone #M94193 (10-P15), N53378-08D: NP-6 Pab rabbit-anti-Hu E B, CCSP-2 antibody) were dissolved at a concentration of 1mg / ml In 0.1mol / L pH9.0 sodium bicarbonate solution.
[0046] 3. Mix the activated biotin solution and the antibody solution to be coupled at a volume ratio of 1:8, and incubate at room temperature for 4 hours.
[0047] Under the condition of 4.4°C, dialyze in 0.05mol / L, pH7.2 PBS for 24h, and change the medium 4 times to remove unbound free biotin.
[0048] 5. Add 0.02% NaN3 to the biotin-bound antibody solution, aliquot them separately, and store them in the dark at ...
Embodiment 3
[0049] Example 3: Application of the liquid chip for parallel detection of colorectal cancer protein markers described in the present invention in clinical detection
[0050] (1) The technical process of using the colorectal cancer protein markers of the present invention to detect protein tumor markers in parallel with liquid-phase chips:
[0051] 1. Take out 500 capture antibody-conjugated microspheres prepared above for each tumor marker, mix them in equal proportions, and distribute them in 96-well plates. Each well contains various capture antibody-conjugated microspheres. For each 500 cells, add 50 μl of serum to be tested and incubate at 37°C for 2 hours.
[0052] 2. Centrifuge at ≥8000×g for 2 minutes, remove the supernatant, add 300 μl of 1% PBS-BSA, vortex for 30 seconds, and seal in a 37°C incubator for 1 hour.
[0053] 3. Centrifuge at ≥8000×g for 2 minutes. Remove the supernatant, add 300 μl PBS-TBN, and vortex for 30 seconds. Centrifuge at ≥8000×g for 2 minute...
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