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Reversible biotinylation of purified proteins for measuring protein-protein interactions

Methods Enzymol. 2020; 
Dwivedi-Agnihotri H, Srivastava A, Shukla AK.
Products/Services Used Details Operation
Proteins, Expression, Isolation and Analysis 2 Reagents for capture and detection of biotinylated proteins Streptavidin beads Magnetic separation rack DTT (Dithiothreitol) Pre-cast or manually prepared acrylamide gels for SDS-PAGE Suitable power supply and SDS-PAGE apparatus Protein molecular weight marker Chemicals for different buffers (Tris–HCl, Glycine, Methanol, Tween- 20, Hydrochloric acid) Coomassie Brilliant blue Suitable power supply and Western blot apparatus for Semi-Dry transfer PVDF membrane for protein transfer Bovine Serum Albumin (For membrane blocking) Streptavidin–horseradish peroxidase antibody (Genscript) Enhanced chemi-luminescence (ECL) reagents Chemi-Doc imaging system 96-well Immuno plates H2SO4 3,3,5,5-Tetramethylbenzidine or TMB substrate Plate reader (Victor 4X multimode plate reader, Perkin Elmer) 2. Get A Quote

摘要

Measuring protein-protein interactions using purified proteins in vitro is one of the most frequently used approach to understand the biochemical and mechanistic details of cellular signaling pathways. Typically, affinity tags are genetically fused to proteins of interest, and they are used to capture and detect them. However, in some cases, fusion of bulky affinity tags might present a significant limitation in these experiments, especially if the regions in close proximity of tags are involved in protein-protein interactions. Here, we present a step-by-step protocol for an alternative approach that involves reversible biotinylation of purified proteins using a simple chemical-conjugation of cleavable biotin m... More

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