Abstract

Antibiotic-resistant infections kill tens of thousands of Americans and cost our nation billions of dollars every year. ?-lactamase enzymes are one of the most common sources of resistance and are capable of quickly evolving the ability to degrade new ?-lactam antibiotics as they are introduced. Surprisingly, many of the mutations that confer ?-lactamases with new functions are far from the enzyme's active site and have little effect on the structure of the active site, as observed by x-ray crystallography. Such non-active site (NAS) mutations also appear frequently in other contexts, such as the evolution of other forms of drug resistance and directed evolution studies. Understanding how NAS mutations allosterically impact distant sites would provide a basis for predicting new forms of drug resistance and designing allosteric drugs to combat diseases like antibiotic-resistant infections. The objective of this proposal is to understand how NAS mutations confer ?- lactamases with activity against new substrates. A predictive understanding of NAS mutations remains elusive because of the ruggedness of proteins' energy landscapes and the great diversity of mechanisms that couple distant residues, including both concerted structural changes and correlations between the dynamics of different residues. These obstacles will be overcome by integrating novel computational methods with in vitro and in vivo experiments to converge on a quantitative understanding of the full spectrum of correlated fluctuations responsible for allosteric coupling. For example, the research team will apply new methods they developed to facilitate comprehensive sampling of proteins' energy landscapes, such as their FAST algorithm for leveraging Markov State Models (MSMs) to efficiently sample conformations with pre-specified features.
In Aim 1, these methods will be used to identify what features of ?-lactamase's structure and dynamics give rise to new activities by comparing models for variants with different activities against the antibiotic cefotaxime.
In aim 2, new methods for identifying both concerted structural changes and correlations between the dynamics of different residues will be developed. These methods will be used to predict new sites where NAS mutations can alter activities of ?-lactamases. To test insights from each aim, mutations will be designed to confer ?- lactamases with new activities. Then experiments will be performed to test 1) whether these mutations have the intended impact on the activities of ?-lactamases and 2) whether the designed variants are capable of protecting bacteria from the target antibiotic. Completion of this work will result in a general framework for understanding allosteric communication that will serve as a basis for future efforts to predict drug resistance, design new antibiotics that allosterically inhibit their targets, and manipulate allostery in other systems.

Public Health Relevance

The mechanisms by which mutations to a protein's sequence confer drug resistance remain poorly understood, especially when these mutations are far from a protein's active site or drug binding site. This proposal aims to identify how these mutations exert allosteric (i.e. long-range) control over distant sites. This understanding will enable us to anticipate and combat drug resistance, in addition to advancing our fundamental understanding of the mechanisms of communication in biological systems.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
1R01GM124007-01
Application #
9361418
Study Section
Macromolecular Structure and Function D Study Section (MSFD)
Program Officer
Wehrle, Janna P
Project Start
2017-09-05
Project End
2022-06-30
Budget Start
2017-09-05
Budget End
2018-06-30
Support Year
1
Fiscal Year
2017
Total Cost
Indirect Cost

  Institution

Name
Washington University
Department
Biochemistry
Type
Schools of Medicine
DUNS #
068552207
City
Saint Louis
State
MO
Country
United States
Zip Code
63130

  Publications

Su, Zhaoming; Wu, Chao; Shi, Liuqing et al. (2018) Electron Cryo-microscopy Structure of Ebola Virus Nucleoprotein Reveals a Mechanism for Nucleocapsid-like Assembly. Cell 172:966-978.e12
Knoverek, Catherine R; Amarasinghe, Gaya K; Bowman, Gregory R (2018) Advanced Methods for Accessing Protein Shape-Shifting Present New Therapeutic Opportunities. Trends Biochem Sci :
Patrick, Garrett J; Fang, Luting; Schaefer, Jacob et al. (2018) Mechanistic Basis for ATP-Dependent Inhibition of Glutamine Synthetase by Tabtoxinine-?-lactam. Biochemistry 57:117-135
Niu, Haixia; Fujiwara, Hideji; di Martino, Orsola et al. (2017) Endogenous retinoid X receptor ligands in mouse hematopoietic cells. Sci Signal 10:
Halstead, Angela M; Kapadia, Chiraag D; Bolzenius, Jennifer et al. (2017) Bladder-cancer-associated mutations in RXRA activate peroxisome proliferator-activated receptors to drive urothelial proliferation. Elife 6:
Zimmerman, Maxwell I; Hart, Kathryn M; Sibbald, Carrie A et al. (2017) Prediction of New Stabilizing Mutations Based on Mechanistic Insights from Markov State Models. ACS Cent Sci 3:1311-1321
Singh, Sukrit; Bowman, Gregory R (2017) Quantifying Allosteric Communication via Both Concerted Structural Changes and Conformational Disorder with CARDS. J Chem Theory Comput 13:1509-1517
Hart, Kathryn M; Ho, Chris M W; Dutta, Supratik et al. (2016) Modelling proteins' hidden conformations to predict antibiotic resistance. Nat Commun 7:12965