TY - JOUR
T1 - Origins of the Mechanochemical Coupling of Peptide Bond Formation to Protein Synthesis
AU - Fritch, Benjamin
AU - Kosolapov, Andrey
AU - Hudson, Phillip
AU - Nissley, Daniel A.
AU - Woodcock, H. Lee
AU - Deutsch, Carol
AU - O'Brien, Edward P.
N1 - Funding Information:
We thank Joseph Larkin for early conversations concerning QM/ MM modeling of peptide bond formation, Nabeel Ahmed for advice on statistical tests, and Fabio Trovato for technical assistance concerning the simulations. This work used the Extreme Science and Engineering Discovery Environment (XSEDE), which is supported by National Science Foundation grant number ACI-1548562. Portions of this research were conducted with Advanced CyberInfrastructure computational resources at The Pennsylvania State University. HLW and PSH acknowledge the support of USF Research Computing (Circe) and the NSF via their Major Research Instrumentation Program (MRI 1531590). NAMD was developed by the Theoretical and Computational Biophysics Group in the Beckman Institute for Advanced Science and Technology at the University of Illinois at Urbana−Champaign. CD acknowledges funding from R01 NIH GM 52302. PSH acknowledges funding support from the Intramural Research Program of the NIH, NHLBI. HLW acknowledges funding from NSF (CHE-1464946). EPO acknowledges funding from Penn State start-up funds, as well as from an NSF CAREER Award (1553291).
Funding Information:
This work used the Extreme Science and Engineering Discovery Environment (XSEDE), which is supported by National Science Foundation grant number ACI-1548562. Portions of this research were conducted with Advanced CyberInfrastructure computational resources at The Pennsylvania State University. HLW and PSH acknowledge the support of USF Research Computing (Circe) and the NSF via their Major Research Instrumentation Program (MRI 1531590). NAMD was developed by the Theoretical and Computational Biophysics Group in the Beckman Institute for Advanced Science and Technology at the University of Illinois at Urbana-Champaign. CD acknowledges funding from R01 NIH GM 52302. PSH acknowledges funding support from the Intramural Research Program of the NIH, NHLBI. HLW acknowledges funding from NSF (CHE-1464946). EPO acknowledges funding from Penn State start-up funds, as well as from an NSF CAREER Award (1553291).
Publisher Copyright:
© 2018 American Chemical Society.
PY - 2018/4/18
Y1 - 2018/4/18
N2 - Mechanical forces acting on the ribosome can alter the speed of protein synthesis, indicating that mechanochemistry can contribute to translation control of gene expression. The naturally occurring sources of these mechanical forces, the mechanism by which they are transmitted 10 nm to the ribosome's catalytic core, and how they influence peptide bond formation rates are largely unknown. Here, we identify a new source of mechanical force acting on the ribosome by using in situ experimental measurements of changes in nascent-chain extension in the exit tunnel in conjunction with all-atom and coarse-grained computer simulations. We demonstrate that when the number of residues composing a nascent chain increases, its unstructured segments outside the ribosome exit tunnel generate piconewtons of force that are fully transmitted to the ribosome's P-site. The route of force transmission is shown to be through the nascent polypetide's backbone, not through the wall of the ribosome's exit tunnel. Utilizing quantum mechanical calculations we find that a consequence of such a pulling force is to decrease the transition state free energy barrier to peptide bond formation, indicating that the elongation of a nascent chain can accelerate translation. Since nascent protein segments can start out as largely unfolded structural ensembles, these results suggest a pulling force is present during protein synthesis that can modulate translation speed. The mechanism of force transmission we have identified and its consequences for peptide bond formation should be relevant regardless of the source of the pulling force.
AB - Mechanical forces acting on the ribosome can alter the speed of protein synthesis, indicating that mechanochemistry can contribute to translation control of gene expression. The naturally occurring sources of these mechanical forces, the mechanism by which they are transmitted 10 nm to the ribosome's catalytic core, and how they influence peptide bond formation rates are largely unknown. Here, we identify a new source of mechanical force acting on the ribosome by using in situ experimental measurements of changes in nascent-chain extension in the exit tunnel in conjunction with all-atom and coarse-grained computer simulations. We demonstrate that when the number of residues composing a nascent chain increases, its unstructured segments outside the ribosome exit tunnel generate piconewtons of force that are fully transmitted to the ribosome's P-site. The route of force transmission is shown to be through the nascent polypetide's backbone, not through the wall of the ribosome's exit tunnel. Utilizing quantum mechanical calculations we find that a consequence of such a pulling force is to decrease the transition state free energy barrier to peptide bond formation, indicating that the elongation of a nascent chain can accelerate translation. Since nascent protein segments can start out as largely unfolded structural ensembles, these results suggest a pulling force is present during protein synthesis that can modulate translation speed. The mechanism of force transmission we have identified and its consequences for peptide bond formation should be relevant regardless of the source of the pulling force.
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U2 - 10.1021/jacs.7b11044
DO - 10.1021/jacs.7b11044
M3 - Article
C2 - 29577725
AN - SCOPUS:85045553329
SN - 0002-7863
VL - 140
SP - 5077
EP - 5087
JO - Journal of the American Chemical Society
JF - Journal of the American Chemical Society
IS - 15
ER -