Abstract
An innovative marriage of techniques, combining the principles of common protein pull-down assays with single-molecule fluorescence microscopy, opens up new ways of visualizing cellular protein complexes. See Article p.484 Analysis of protein interactions is crucial for understanding cellular function and regulation. Here, Taekjip Ha and colleagues develop a novel method for elucidating the identity and stoichiometry of protein complexes from cells and tissues at single-molecule resolution. The method, called single molecule pull-down or SiMPull, can discriminate between multiple association states of a protein, and simultaneously allows determination of complex stoichiometry through photobleaching step analysis. The potential of the assay is demonstrated in a variety of contexts, including endogenous proteins from tissue extracts, organelles and membrane proteins.
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