High-flux screening cell model of alpha1-AR subtype selective antagonist, and construction method and application thereof
A cell model, 1-AR technology, applied to cells modified by introducing foreign genetic material, biochemical equipment and methods, recombinant DNA technology, etc., can solve the problem of poor screening effect of anti-benign prostatic hyperplasia drugs, etc. To achieve the effect of efficient, fast and rapid screening of the method
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Embodiment 1
[0037] alpha 1 -Building process of high-throughput screening model for AR subtype-selective antagonists
[0038] S1. Preservation and extraction of plasmids (pGL4.29[luc2P / CRE / Hygro], pGL4.74[hRluc / TK], EX-A0967-M29, EX-Y3321-M29, EX-Y2008-M29).
[0039] S11. Plasmid transformation and storage: Transfer 1 μL of the above plasmid to the bottom of a 1.5 mL centrifuge tube for ice bath, add to 200 μL of competent cells (DH5α), mix well, and place in ice bath for 30 minutes. Heat shock at 42°C for 40s and ice bath for 3min. Add 400 μL of S.O.C medium, shake culture at 37°C for 1 hour, take 50 μL and spread it on the surface of the solid medium plate containing 100ug / mL ampicillin. Cultivate overnight at 37°C, pick a single clone and inoculate it into 500 μL LB liquid medium, culture on a shaker at 37°C for 6 hours, add resistant glycerol containing 100 μg / mL ampicillin, and the final concentration of glycerol is 15-25%.
[0040] S12. Strain cultivation and plas...
Embodiment 2
[0059] In order to determine the suitable reporter gene in the screening method of the present invention, the present invention studies the response of five response factors directly or indirectly related to α1-ARs, the specific method is as follows:
[0060] Will α 1 -ARs (ADRA1A, ADRA1B and ADRA1D) were co-transfected with the reporter gene and the internal reference plasmid (hRluc-TK) respectively. Negative control and blank control were used for drug addition to investigate the fluorescence induced by the reporter gene to phenylephrine in the co-transfection system. The influence of signal ratio, in which the reporter gene selects 5 main response elements that are directly or indirectly related to α1-ARs: cyclic adenosinase response element (CRE), serum response element (SRE) and activin-1 response element ( AP-1), nuclear factor-кB (NF-кB-RE) and nuclear factor of activated T cells (NFAT-RE), respectively inserted into the firefly luciferase vector (luc2P) to co...
Embodiment 3
[0061] Example 3 Scale Selection of Reporting Components
[0062] The difference in the ratio of the reporter element plasmid has an important influence on the difference in luciferase expression value caused by receptor signal transduction after adding phenylephrine stimulation. In order to ensure the stable and optimal expression of luciferase on the screening platform, the ratio of ADRA1D, reporter gene Luc2P-CRE, and internal reference plasmid (hRluc-TK) was optimized, other conditions and methods were fixed, and the ratio of reporter gene and internal reference plasmid was changed. , to detect differences in luciferase expression intensity at different doses. Such as figure 2 As shown, the eukaryotic expression plasmid, reporter gene, and internal reference plasmid are respectively 1:1:1; 1:10:1; 1:50:1; 1:100:1; 10:100:1; 50:100:1 ; 100:100:1 for co-transfection, the results showed ( figure 2 ), according to the plasmid ratio of 1:1:1, a better signal-to-noise r...
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