Stochastic but Highly Coordinated Protein Unfolding and Translocation by the ClpXP Proteolytic Machine

Author(s)

Cordova, Juan Carlos; Aubin-Tam, Marie-Eve; Lang, Matthew J.; Olivares, Adrian O.; Shin, Yongdae; Calmat, Stephane Geraldine Michele; Schmitz, Karl Robert; Baker, Tania; Sauer, Robert T.; Stinson, Benjamin Michael; ... Show more Show less

Abstract

ClpXP and other AAA+ proteases recognize, mechanically unfold, and translocate target proteins into a chamber for proteolysis. It is not known whether these remarkable molecular machines operate by a stochastic or sequential mechanism or how power strokes relate to the ATP-hydrolysis cycle. Single-molecule optical trapping allows ClpXP unfolding to be directly visualized and reveals translocation steps of ∼1–4 nm in length, but how these activities relate to solution degradation and the physical properties of substrate proteins remains unclear. By studying single-molecule degradation using different multidomain substrates and ClpXP variants, we answer many of these questions and provide evidence for stochastic unfolding and translocation. We also present a mechanochemical model that accounts for single-molecule, biochemical, and structural results for our observation of enzymatic memory in translocation stepping, for the kinetics of translocation steps of different sizes, and for probabilistic but highly coordinated subunit activity within the ClpX ring.

Date issued

2014-07

URI

http://hdl.handle.net/1721.1/106303

Department

Massachusetts Institute of Technology. Department of Biology
Massachusetts Institute of Technology. Department of Mechanical Engineering

Journal

Cell

Publisher

Elsevier

Citation

Cordova, Juan Carlos et al. “Stochastic but Highly Coordinated Protein Unfolding and Translocation by the ClpXP Proteolytic Machine.” Cell 158.3 (2014): 647–658.

Version: Author's final manuscript

ISSN

0092-8674

1097-4172