Abstract

Proper cellular function requires efficient folding of cellular proteins. In the cell, protein folding starts co-translationally, concomitantly with protein synthesis by the ribosome, following pathways that can be distinct from the refolding of full-length proteins in vitro. The average, bulk translation rate in E. coli is -20 aa/sec, but this rate can vary by more than an order of magnitude for the translation of specific mRNA sequences. Recent results have highlighted that altering the translation rate of small portions of some genes can significantly affect the folding efficiency of the encoded protein (correct folding versus misfolding and aggregation, or degradation), or alter the partitioning between two alternative folded structures. Yet despite the potential impact of local translation rate on protein biogenesis in vivo, the interactions between the ribosome and mRNA and/or nascent chain sequences that control local translation rate remain opaque. Nor do we know what fraction of proteins in the proteome has co-translational folding mechanisms that are significantly affected by altered translation rate. The PIs of this proposal have constructed a network to span their established expertise in genetics, molecular biology, genomics, biochemistry, biophysics, and organic, analytical and physical chemistry, creating a team uniquely suited to tackle three significant outstanding questions regarding the mechanisms and outcomes of altered translation rate in E. coli. Our network will determine: (1) What specific features of mRNA and/or nascent chain sequences shape absolute local translation rate in vivo, and by what mechanisms? (2) What proteins in the proteome are most susceptible to aggregation or degradation when translation rate is altered? (3) To what extent does translational pausing alter the conformation of the ribosome and/or its interactions with other proteins in vivo? Taken together, results from this proposal will represent crucial steps towards a comprehensive picture of translation rate control in E. coli, and the effects of altered translation rate on protein biogenesis, including the heterologous expression of human proteins.

Public Health Relevance

RELEVENCE: The rate of protein synthesis is not uniform, but we do not fully understand why some sequences are translated more slowly than others. Altering local translation rate can affect protein folding, and hence cell function. We will develop new approaches to measure local translation rates and the mechanisms that determine these rates, and identify proteins whose folding is most affected by translation rate differences.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Specialized Center--Cooperative Agreements (U54)
Project #
5U54GM105816-03
Application #
8853885
Study Section
Special Emphasis Panel (ZGM1-CBB-0 (MI))
Program Officer
Willis, Kristine Amalee
Project Start
2013-06-10
Project End
2018-04-30
Budget Start
2015-05-01
Budget End
2016-04-30
Support Year
3
Fiscal Year
2015
Total Cost
$674,636
Indirect Cost
$64,451

  Institution

Name
University of Notre Dame
Department
Chemistry
Type
Schools of Arts and Sciences
DUNS #
824910376
City
Notre Dame
State
IN
Country
United States
Zip Code
46556

  Publications

Riback, Joshua A; Katanski, Christopher D; Kear-Scott, Jamie L et al. (2017) Stress-Triggered Phase Separation Is an Adaptive, Evolutionarily Tuned Response. Cell 168:1028-1040.e19
Byun, Hyewon; Das, Poulami; Yu, Houqing et al. (2017) Mouse Mammary Tumor Virus Signal Peptide Uses a Novel p97-Dependent and Derlin-Independent Retrotranslocation Mechanism To Escape Proteasomal Degradation. MBio 8:
Yu, Houqing; Singh Gautam, Amit K; Wilmington, Shameika R et al. (2016) Conserved Sequence Preferences Contribute to Substrate Recognition by the Proteasome. J Biol Chem 291:14526-39
Bhattacharyya, Sucharita; Renn, Jonathan P; Yu, Houqing et al. (2016) An assay for 26S proteasome activity based on fluorescence anisotropy measurements of dye-labeled protein substrates. Anal Biochem 509:50-59
Yu, Houqing; Kago, Grace; Yellman, Christopher M et al. (2016) Ubiquitin-like domains can target to the proteasome but proteolysis requires a disordered region. EMBO J 35:1522-36
Martinez-Fonts, Kirby; Matouschek, Andreas (2016) A Rapid and Versatile Method for Generating Proteins with Defined Ubiquitin Chains. Biochemistry 55:1898-908
Li, Sujun; Dabir, Aditi; Misal, Santosh A et al. (2016) Impact of Amidination on Peptide Fragmentation and Identification in Shotgun Proteomics. J Proteome Res 15:3656-3665
Jacobson, Giselle N; Clark, Patricia L (2016) Quality over quantity: optimizing co-translational protein folding with non-'optimal' synonymous codons. Curr Opin Struct Biol 38:102-10
Clark, Patricia L (2016) How to Build a Complex, Functional Propeller Protein, From Parts. Trends Biochem Sci 41:290-292
Mohammad, Fuad; Woolstenhulme, Christopher J; Green, Rachel et al. (2016) Clarifying the Translational Pausing Landscape in Bacteria by Ribosome Profiling. Cell Rep 14:686-694

Showing the most recent 10 out of 24 publications