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- 详细信息
- 技术资料
- 规格:
96T
| Catalog | Components | 96tests | 480tests |
| A001-214 | Human PD-L1 | 25 μg | 125 μg |
| A002-214 | Human PD-1-Biotin | 5 μg | 25 μg |
| A003-214 | Streptavidin-HRP | 5 μg | 25 μg |
| PD1-NA001 | Anti-PD-1 Neutralizing Antibody | 20 μg | 100 μg |
Introduction:
Immune checkpoint pathway is a focal point of today’s cancer research. PD-1 is one of the best characterized checkpoint proteins. The binding between PD-1 and its ligand PD-L1 suppresses T-cell activation and allows cancer cells to escape from body’s immune surveillance. Therefore, the pharmaceutical inhibition of PD-1 or its ligand has been considered a promising strategy by many oncologists.
Reconstitution:
See Certificate of Analysis for details of reconstitution instruction and specific concentration.
Storage:
See Certificate of Analysis for details of storage conditions.
Be sure to store each component at the proper tempe rature upon arrival
Avoid freeze/thaw cycles upon reconstituted.
Application:
This pair is useful for screening for inhibitors of human PD-1 binding to human PD-L1.
Description:
This inhibitor screening ELISA pair is designed to facilitate the identification and characterization of new PD-1 pathway inhibitors. The assay takes advantage of our in house-developed binding of biotinylated human PD-1 to immobilized human PD-L1 in a functional ELISA assay, and employs a simple colorimetric sandwich ELISA platform. Briefly, we provide you with a human PD-1-Biotin protein, a human PD-L1 protein, an anti-PD-1 neutralizing antibody (as method verified Std.), and streptavidin-HRP reagent. Your experiment will include 4 simple steps: a) Coat the plate with human PD-L1. b) Add your molecule of interest to the tests. c) Add Human PD-1-Biotin to bind the coated human PD-L1. d) Add Streptavidin-HRP followed by TMB or other colorimetric HRP substrate. Finally, the ability of your compound to inhibit PD-1 : PD-L1 binding will be determined by comparing OD readings among different experimental groups.
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