Ultrafast folding kinetics and cooperativity of villin headpiece in single-molecule force spectroscopy

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Abstract

In this study we expand the accessible dynamic range of single-molecule force spectroscopy by optical tweezers to the microsecond range by fast sampling. We are able to investigate a single molecule for up to 15 min and with 300-kHz bandwidth as the protein undergoes tens of millions of folding/unfolding transitions. Using equilibrium analysis and autocorrelation analysis of the time traces, the full energetics as well as real-time kinetics of the ultrafast folding of villin headpiece 35 and a stable asparagine 68 alanine/lysine 70 methionine variant can be measured directly. We also performed Brownian dynamics simulations of the response of the bead-DNA system to protein-folding fluctuations. All key features of the force-dependent deflection fluctuations could be reproduced: SD, skewness, and autocorrelation function. Our measurements reveal a difference in folding pathway and cooperativity between wild-type and stable variant of headpiece 35. Autocorrelation force spectroscopy pushes the time resolution of single-molecule force spectroscopy to 10 μs thus approaching the timescales accessible for all atom molecular dynamics simulations.

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CITATION STYLE

APA

Žoldák, G., Stigler, J., Pelz, B., Li, H., & Rief, M. (2013). Ultrafast folding kinetics and cooperativity of villin headpiece in single-molecule force spectroscopy. Proceedings of the National Academy of Sciences of the United States of America, 110(45), 18156–18161. https://doi.org/10.1073/pnas.1311495110

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