Abstract

The ClC family of chloride channels and transporters play important physiological roles. Mutations in ClC family proteins are associated with an array of diseases, some of which are caused by protein misfolding. Thus, it is important to understand how these protein fold. Yet the folding of ClC family proteins presents a formidable challenge, for both biology and experiment. Not only are they large membrane proteins, but they have a remarkably complex topology with many helices that insert only part way into the bilayer and then loop back out, leaving considerable polar surfaces in the center of the bilayer. How proteins like this can fold in the apolar bilayer remains unknown and largely unexamined. Using a new single molecule forced unfolding technique we developed in the prior grant period, we made some surprising discoveries regarding the folding of the ClC antiporter from E. coli that we now propose to investigate more deeply. In particular, it appears that the protein folds in two domains that would require plunging polar moieties into the apolar bilayer. Why would the protein be designed to fold in this manner and how might it be accomplished? To address these issues we propose the following aims:
Aim I : Structure of isolated ClC domains. We will investigate the structures of the domains with polar exposed surfaces in isolation and how they adapt to the bilayer environment.
Aim II : How do lipid properties affect the stability of the isolated domains? To gain insight into the interaction of the protein and lipids during unfolding and folding, we will examine the effects of different lipids on the energetics of domain separation.
Aim III : Can separate folding of the domains increase folding efficiency? Is there evidence for N- to C-terminal folding? We hypothesize that dividing the folding of ClC-ec into two units simplifies the folding of such a large complex protein. As the protein emerges from the translocon, the N-terminal domain may commence folding, reducing options for the C-terminal domain and possibly templating C-terminal domain folding. To test this hypothesis we will examine the folding efficiency and folding kinetics of the individual domains by themselves and in the presence of the other domain. Our work will map the folding energetics and pathway for arguably the most complex protein ever studied at this level; provide insight into the folding of the large number of membrane proteins with re-entrant helices; and provide new ideas for intervening in membrane protein folding diseases.

Public Health Relevance

Proteins often fold up into a unique structure that is essential for its biological role, and disease can occur if the folding process is disrupted by mutation or other aberrant physiological processes. We are working to understand how the many proteins that float in cell membranes manage to assemble so that we can ultimately learn how to intervene in folding diseases.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM063919-18
Application #
9723124
Study Section
Biochemistry and Biophysics of Membranes Study Section (BBM)
Program Officer
Preusch, Peter
Project Start
2001-08-01
Project End
2022-08-31
Budget Start
2019-09-01
Budget End
2020-08-31
Support Year
18
Fiscal Year
2019
Total Cost
Indirect Cost

  Institution

Name
University of California Los Angeles
Department
Chemistry
Type
Schools of Arts and Sciences
DUNS #
092530369
City
Los Angeles
State
CA
Country
United States
Zip Code
90095

  Publications

Lu, Peilong; Min, Duyoung; DiMaio, Frank et al. (2018) Accurate computational design of multipass transmembrane proteins. Science 359:1042-1046
Jefferson, Robert E; Min, Duyoung; Corin, Karolina et al. (2018) Applications of Single-Molecule Methods to Membrane Protein Folding Studies. J Mol Biol 430:424-437
Min, Duyoung; Jefferson, Robert E; Qi, Yifei et al. (2018) Unfolding of a ClC chloride transporter retains memory of its evolutionary history. Nat Chem Biol 14:489-496
Cao, Zheng; Hutchison, James M; Sanders, Charles R et al. (2017) Backbone Hydrogen Bond Strengths Can Vary Widely in Transmembrane Helices. J Am Chem Soc 139:10742-10749
Woodall, Nicholas B; Hadley, Sarah; Yin, Ying et al. (2017) Complete topology inversion can be part of normal membrane protein biogenesis. Protein Sci 26:824-833
Cheng, Xi; Kim, Jin-Kyoung; Kim, Yangmee et al. (2016) Molecular dynamics simulation strategies for protein-micelle complexes. Biochim Biophys Acta 1858:1566-72
Nam, Hyun-Jun; Kim, Inhae; Bowie, James U et al. (2015) Metazoans evolved by taking domains from soluble proteins to expand intercellular communication network. Sci Rep 5:9576
Woodall, Nicholas B; Yin, Ying; Bowie, James U (2015) Dual-topology insertion of a dual-topology membrane protein. Nat Commun 6:8099
Min, Duyoung; Jefferson, Robert E; Bowie, James U et al. (2015) Mapping the energy landscape for second-stage folding of a single membrane protein. Nat Chem Biol 11:981-7
Cao, Zheng; Bowie, James U (2014) An energetic scale for equilibrium H/D fractionation factors illuminates hydrogen bond free energies in proteins. Protein Sci 23:566-75

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