Abstract

The process through which the two-subunit ribosome assembles at the start codon of an mRNA to initiate protein synthesis is one of the most fundamental and highly regulated steps of gene expression. As such, initiation serves as the target of numerous small-molecule antibiotics and cellular pathogens. Moreover, deregulation of initiation is causally linked to viral infections and tumorigenesis in humans. Given all of this, studies of the molecular mechanism of initiation hold great promise for the identification and characterization of mechanistic steps that can serve as targets for the development of next-generation antibiotics and other small- molecule, anti-viral, and anti-cancer drugs that act by modulating translation initiation. Despite their promise for molecular medicine, mechanistic studies of initiation remain incredibly challenging. This is primarily because initiation is an extraordinarily dynamic, multi-step process that proceeds through a large number of short-lived intermediate states that are very difficult to observe and characterize using conventional approaches. During initiation, a set of essential initiation factors (IFs) transiently interact with both ribosomal subunits and a specialized initiator tRNA in order to guide their assembly at the start codon of the mRNA to be translated. Although evidence suggests that the IFs, ribosomal subunits, and tRNA undergo functionally important structural rearrangements during this process, very few of these rearrangements have been directly observed and/or characterized, and for those that have, it has been at very low resolution. The long-term goals of this project are to use powerful combinations of reagents and techniques that are uniquely available in our and our collaborators? laboratories to overcome the challenges associated with mechanistic studies of initiation. Specifically, we will use state-of-the-art single-molecule fluorescence microscopy and cryogenic electron microscopy (cryo-EM), including a pioneering, time-resolved cryo-EM approach developed by our collaborator, Dr. Joachim Frank, to directly observe and characterize the dynamics of initiation. These studies will be enabled by a new approach that we have developed for introducing fluorophores into ribosomes at positions that are highly desirable, but that have thus far remained out of reach.
In Aim 1, we will investigate the mechanism through which bacterial IF2 transiently binds to a ribosomal initiation complex (IC) based on the small, 30S, ribosomal subunit (30S IC); determines whether the 30S IC is carrying an accurately selected initiator tRNA that is properly base-paired to a correctly selected start codon; and, if so, recruits and facilitates joining of the large, 50S, ribosomal subunit to the 30S IC.
In Aim 2, we will investigate the mechanism through which bacterial IF3 and IF1 ensure the accuracy with which the start codon is selected during initiation.
In Aim 3, we will extend our studies to investigate the mechanism of eukaryotic translation initiation, focusing our attention on eukaryotic-specific aspects of the mechanism through which the eukaryotic homolog of IF2, eukaryotic IF5B (eIF5B), regulates subunit joining during eukaryotic initiation.

Public Health Relevance

) The essential task of synthesizing all the proteins encoded in an organism?s DNA is executed by the ribosome and its associated translation machinery (TM), the bacterial variants of which serve as the targets of over half of the antibacterial drugs that are currently in clinical use. Moreover, loss of control over the process through which the human eukaryotic TM synthesize proteins has been shown to be causative for many human diseases, including numerous viral infections and cancers. Using a powerful combination of reagents approaches that are unique to the applicant?s and collaborator?s laboratories, this proposal will elucidate fundamental steps in the process of protein synthesis by the bacterial and eukaryotic TMs that have the potential to serve as targets for the development of next-generation antibacterial drugs as well as other small- molecule drugs that can be used to treat viral infections, cancers, and other human diseases.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
3R01GM084288-11S1
Application #
10135551
Study Section
Special Emphasis Panel (ZRG1)
Program Officer
Reddy, Michael K
Project Start
2008-12-01
Project End
2023-07-31
Budget Start
2020-08-01
Budget End
2021-07-31
Support Year
11
Fiscal Year
2020
Total Cost
Indirect Cost

  Institution

Name
Columbia University (N.Y.)
Department
Chemistry
Type
Graduate Schools
DUNS #
049179401
City
New York
State
NY
Country
United States
Zip Code
10027

  Publications

Subramanyam, Shyamal; Kinz-Thompson, Colin D; Gonzalez Jr, Ruben L et al. (2018) Observation and Analysis of RAD51 Nucleation Dynamics at Single-Monomer Resolution. Methods Enzymol 600:201-232
Kinz-Thompson, Colin D; Gonzalez Jr, Ruben L (2018) Increasing the Time Resolution of Single-Molecule Experiments with Bayesian Inference. Biophys J 114:289-300
Caban, Kelvin; Pavlov, Michael; Ehrenberg, Måns et al. (2017) A conformational switch in initiation factor 2 controls the fidelity of translation initiation in bacteria. Nat Commun 8:1475
Kinz-Thompson, C D; Bailey, N A; Gonzalez Jr, R L (2016) Precisely and Accurately Inferring Single-Molecule Rate Constants. Methods Enzymol 581:187-225
Greenfeld, Max; van de Meent, Jan-Willem; Pavlichin, Dmitri S et al. (2015) Single-molecule dataset (SMD): a generalized storage format for raw and processed single-molecule data. BMC Bioinformatics 16:3
Ruehle, Marisa D; Zhang, Haibo; Sheridan, Ryan M et al. (2015) A dynamic RNA loop in an IRES affects multiple steps of elongation factor-mediated translation initiation. Elife 4:
Caban, Kelvin; Gonzalez Jr, Ruben L (2015) The emerging role of rectified thermal fluctuations in initiator aa-tRNA- and start codon selection during translation initiation. Biochimie 114:30-8
Thompson, Colin D Kinz; Sharma, Ajeet K; Frank, Joachim et al. (2015) Quantitative Connection between Ensemble Thermodynamics and Single-Molecule Kinetics: A Case Study Using Cryogenic Electron Microscopy and Single-Molecule Fluorescence Resonance Energy Transfer Investigations of the Ribosome. J Phys Chem B 119:10888-10901
Wang, Jiangning; Caban, Kelvin; Gonzalez Jr, Ruben L (2015) Ribosomal initiation complex-driven changes in the stability and dynamics of initiation factor 2 regulate the fidelity of translation initiation. J Mol Biol 427:1819-34
Pereira, Sandro F F; Gonzalez Jr, Ruben L; Dworkin, Jonathan (2015) Protein synthesis during cellular quiescence is inhibited by phosphorylation of a translational elongation factor. Proc Natl Acad Sci U S A 112:E3274-81

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