The cofactor-dependent folding mechanism of Drosophila cryptochrome revealed by single-molecule pulling experiments

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作者
Sahar Foroutannejad
Lydia L. Good
Changfan Lin
Zachariah I. Carter
Mahlet G. Tadesse
Aaron L. Lucius
Brian R. Crane
Rodrigo A. Maillard
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[1] Georgetown University,Department of Chemistry
[2] Cornell University,Department of Chemistry & Chemical Biology
[3] University of Alabama at Birmingham,Department of Chemistry
[4] Georgetown University,Department of Mathematics and Statistics
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The link between cofactor binding and protein activity is well-established. However, how cofactor interactions modulate folding of large proteins remains unknown. We use optical tweezers, clustering and global fitting to dissect the folding mechanism of Drosophila cryptochrome (dCRY), a 542-residue protein that binds FAD, one of the most chemically and structurally complex cofactors in nature. We show that the first dCRY parts to fold are independent of FAD, but later steps are FAD-driven as the remaining polypeptide folds around the cofactor. FAD binds to largely unfolded intermediates, yet with association kinetics above the diffusion-limit. Interestingly, not all FAD moieties are required for folding: whereas the isoalloxazine ring linked to ribitol and one phosphate is sufficient to drive complete folding, the adenosine ring with phosphates only leads to partial folding. Lastly, we propose a dCRY folding model where regions that undergo conformational transitions during signal transduction are the last to fold.
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