Method for carrying out enzyme-linked immunoadsorption detection on integral zebra fish and application thereof
An enzyme-linked immunosorbent adsorption and zebrafish technology, which is applied in the direction of biological testing, material inspection products, etc., can solve the problems of long experimental cycle, complicated operation, and many false positive results, and achieve stable experimental results, increase screening speed, and broad application prospects Good results
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Embodiment 1
[0172] Determination of the optimal developmental stage of zebrafish when the compound of Example 1 is processed
[0173] Embryo collection
[0174] In the early morning, 5 pairs of zebrafish were taken, freely combined and divided into 5 groups to mate and hatch embryos, and 1200 zebrafish were collected, the sediment was sucked out, put into the incubation solution, and incubated in a 28°C incubator. In the middle, take out the white embryo (dead) in time to prevent the water quality from deteriorating, because the zebrafish obtains nutrients through the yolk during this period, so no other nutrients are needed.
[0175] drug treatment
[0176] The zebrafish were divided into 7 experimental groups, which were 1 day, 2 days, 3 days, 4 days, 5 days, 6 days, and 7 days after fertilization. Each experimental group was divided into three groups, blank group, 0.1% dimethyl sulfoxide (DMSO) negative control group and experimental treatment group (50 μ M staurosporine (staurospori...
Embodiment 2
[0184]Embodiment 2 compound processes the mensuration of optimal length of time
[0185] Embryo collection
[0186] In the early morning, 5 pairs of zebrafish were taken, freely combined and divided into 5 groups to mate and hatch embryos, and 1200 zebrafish were collected, the sediment was sucked out, put into the incubation solution, and incubated in a 28°C incubator. In the middle, take out the white embryo (dead) in time to prevent the water quality from deteriorating, because the zebrafish obtains nutrients through the yolk during this period, so no other nutrients are needed.
[0187] drug treatment
[0188] Zebrafish were divided into five experimental groups, each group including blank group, treatment group (50 μM staurosporine (staurosporine), 0.1% dimethyl sulfoxide (DMSO) dissolved) and negative control group (0.1% dimethyl sulfoxide (DMSO) sulfoxide (DMSO)). The experimental groups were treated 2 days after zebrafish fertilization, and the treatment time was 6 ...
Embodiment 3
[0196] The detection of embodiment 3 drug genotoxicity
[0197] Embryo collection
[0198] In the early morning, 10 pairs of zebrafish were taken, freely combined and divided into 10 groups to mate and hatch embryos, 1200 zebrafish were collected, the sediment was sucked out, put into the incubation solution, and incubated in a 28°C incubator. In the middle, take out the white embryo (dead) in time to prevent the water quality from deteriorating, because the zebrafish obtains nutrients through the yolk during this period, so no other nutrients are needed.
[0199] drug treatment
[0200] The zebrafish were divided into eight experimental groups, respectively 0.1, 1, 10, 100, 1000 μ M genotoxic drug cisplatin (cisplatin), and then dissolved in the hatching solution according to the above concentration; the blank group was no treatment, 0.1% di Methyl sulfoxide (DMSO) negative control group, 50 μM staurosporine (staurosporine) positive control group that can cause genotoxicity...
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Abstract
Description
Claims
Application Information
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