Abstract

All proteins sample a diverse array of conformations (folded, unfolded, and excited states) with differing free energies and dynamics depending on the environmental conditions. A protein?s primary sequence encodes more than just the native structure; it encodes the entire energy landscape ? an ensemble of conformations whose energetics and dynamics are finely tuned and modulated. The goal of this proposal is a quantitative and predictive understanding of the relationship between sequence and the landscape, together with an understanding of how a protein?s environment modulates this landscape. A major hurdle in going from sequence to function is our lack of understanding of the non-native regions of the landscape. High-energy conformations are important for directing the stability and folding of a protein, and modulations of this ensemble play a role in misfolding, protein signaling, catalytic activity, and allostery. While many sequences can encode the same structure, their function and dynamics can vary dramatically ? due to changes in the landscape. Small variations in a sequence can have effects that range from undetectable to pathological. Soon we will have access to thousands of human genomes, and without an ability to interpret variation, the potential of these data to impact medicine and human health will not be fully appreciated. The experiments outlined here will focus on how modulations in the cellular environment (the ribosome, post-translational modifications and co-translational folding) affect a protein?s energy landscape as well as new approaches to investigate the effect of sequence variation on these landscapes.
Aim 1. How do cellular components (the ribosome and ubiquitination) modulate the energy landscape? a. Determine the effect of ubiquitination on the energy landscape of target proteins. b. Determine the effects of the ribosome on the energy landscape of ribosome-bound nascent chains (RNCs), monitoring kinetics and hydrogen exchange.
Aim 2 : Biophysical studies of co-translational folding a. Determine the role of topology by studying the co-translational folding of circular permutants of HaloTag. b. Monitor protein folding in complex environments using X-ray hydroxyl radical footprinting (XF/MS). c. Probe the temporal coordination between translation and nascent chain folding using single-molecule fluorescence in zero-mode waveguides.
Aim 3 : ASR studies to probe the sequence determinants of protein landscapes a. Probing the rate-limiting step in protein folding by investigating a family containing kinetically stable and thermodynamically stable proteins. b. ASR analysis on the alpha-lytic protease family.

Public Health Relevance

The primary sequence of a protein specifies the entire energy landscape, which describes all of a protein? conformations and dynamics, and is critical for proper function and cellular health. Small changes in sequence and environment can have effects that range from undetectable to pathological; without our ability to interpret these effects, the impact of the explosion in human genome sequences will never be realized. The goal of this proposal is a molecular, quantitative, and predictive understanding of the relationship between sequence and the energy landscape, together with a predictive understanding of how the environment modulates this landscape.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM050945-27
Application #
10023263
Study Section
Macromolecular Structure and Function B Study Section (MSFB)
Program Officer
Lyster, Peter
Project Start
1994-05-01
Project End
2023-07-31
Budget Start
2020-08-01
Budget End
2021-07-31
Support Year
27
Fiscal Year
2020
Total Cost
Indirect Cost

  Institution

Name
University of California Berkeley
Department
Biochemistry
Type
Schools of Arts and Sciences
DUNS #
124726725
City
Berkeley
State
CA
Country
United States
Zip Code
94710

  Publications

Lim, Shion A; Marqusee, Susan (2018) The burst-phase folding intermediate of ribonuclease H changes conformation over evolutionary history. Biopolymers 109:e23086
Samelson, Avi J; Bolin, Eric; Costello, Shawn M et al. (2018) Kinetic and structural comparison of a protein's cotranslational folding and refolding pathways. Sci Adv 4:eaas9098
Zhang, Yongli; Ha, Taekjip; Marqusee, Susan (2018) Editorial Overview: Single-Molecule Approaches up to Difficult Challenges in Folding and Dynamics. J Mol Biol 430:405-408
Guinn, Emily J; Tian, Pengfei; Shin, Mia et al. (2018) A small single-domain protein folds through the same pathway on and off the ribosome. Proc Natl Acad Sci U S A 115:12206-12211
Guinn, Emily J; Marqusee, Susan (2018) Exploring the Denatured State Ensemble by Single-Molecule Chemo-Mechanical Unfolding: The Effect of Force, Temperature, and Urea. J Mol Biol 430:450-464
Lim, Shion An; Bolin, Eric Richard; Marqusee, Susan (2018) Tracing a protein's folding pathway over evolutionary time using ancestral sequence reconstruction and hydrogen exchange. Elife 7:
Hamadani, Kambiz M; Howe, Jesse; Jensen, Madeleine K et al. (2017) An in vitro tag-and-modify protein sample generation method for single-molecule fluorescence resonance energy transfer. J Biol Chem 292:15636-15648
Samelson, Avi J; Jensen, Madeleine K; Soto, Randy A et al. (2016) Quantitative determination of ribosome nascent chain stability. Proc Natl Acad Sci U S A 113:13402-13407
Wheeler, Lucas C; Lim, Shion A; Marqusee, Susan et al. (2016) The thermostability and specificity of ancient proteins. Curr Opin Struct Biol 38:37-43
Lim, Shion A; Hart, Kathryn M; Harms, Michael J et al. (2016) Evolutionary trend toward kinetic stability in the folding trajectory of RNases H. Proc Natl Acad Sci U S A 113:13045-13050

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