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ATAT1, GST-tag Recombinant
面议ATF2, GST-Tag Recombinant
面议GCN5 (727-837), His-tag Recombinant
面议GCN5 (KAT2A), FLAG-tag Recombinant
面议p300 (KAT3B), His-GST-tag Recombinant
面议ACHE, His-Tag Recombinant
面议APAF1, His-tag, FLAG-tag Recombinant
面议BCL-2, His-Tag Recombinant
面议BCL2A1, His-Tag Recombinant
面议BCL2L10, His-Tag Recombinant
面议Caspase6, His-tag Recombinant
面议Caspase7, His-tag Recombinant
面议The KRAS(G12V) Nucleotide Exchange Assay is a homogeneous assay designed for the screening and profiling of KRAS(G12V) antagonists/inhibitors by using BODIPY®-GDP to monitor the GDP or GTP binding status. The kit can be used with two different protocols for greater flexibility, either titrating the inhibitor at a fixed GTP concentration or titrating the GTP at a fixed inhibitor concentration.
BODIPY® FL-GDP is a mixed isomer in which the fluorophore has been attached to the 2’ or 3’ position of the ribose ring via a linker. It is a green-fluorescent dye with similar excitation and emission to fluorescein or Alexa Fluor™ 488, characterized by a high extinction coefficient and high quantum yield and is relatively insensitive to pH changes. The dye has an excited-state lifetime of 5 nanoseconds or longer.
Assay Principle Illustration: KRAS is activated upon binding GTP, when it undergoes a conformational change. KRAS then returns to a GDP-bound inactive state following the hydrolysis of GTP to GDP. In this assay, KRAS is pre-loaded with fluorescent BODIPY®-GDP and therefore is inactive. Adding GTP in the presence of EDTA displaces BODIPY®-GDP because KRAS affinity for GTP is greater than its affinity for GDP. The fluorescence intensity decreases as the BODIPY®-GDP is displaced. Several KRAS inhibitors lock KRAS in the (inactive) GDP-bound conformation and prevent GDP/GTP exchange. In this scenario the fluorescence intensity increases with drug concentration as more BODIPY®-GDP remains bound to KRAS.