Abstract

This supplement will critically update the instrumentation available for all aspects of the parent grant, Riboswitch mechanism unraveled at the single molecule level, as well as all 3.5 NIGMS R01 grants of the PI that are currently pending conversion into a single R35 MIRA award, entitled The RNA nanomachines of gene expression dissected at the single molecule level. The most critical aspects of the proposed instrumentation, the ONI Nanoimager S, are its versatility, turnkey readiness, and ease of use. These features will dramatically facilitate access by the diverse group of postdoctoral fellows, graduate students and undergraduate students in the PI?s group to a plethora of single molecule fluorescence microscopy tools. In turn, these tools are leveraged directly by the parent grant, which is focused on dissecting the mechanisms of the nanoscale RNA machines of gene expression at the single molecule level. Building on our group?s 20-year expertise in this space, we aim to: 1.) Apply our established mechanistic enzymology approaches to an ever broader set of RNAs involved in regulating transcription, translation and splicing, seizing the opportunities arising from the continuing discoveries of new functional RNAs. 2.) Push the limits of our approaches to be able to probe increasingly complex biological contexts and mechanisms since unexpected discoveries often await where individual RNA nanomachines interact. In pursuit of these aims, we will address the unifying hypothesis that dynamic RNA structures are a major determinant of the outcomes of gene expression, as exemplified by the fact that nascent RNA structure has a significant impact on both transcription and translation in the form of regulatory riboswitches embedded near the 5? ends of bacterial mRNAs. Exemplifying the power of our scientific approach to address our hypothesis, we recently combined single-molecule, biochemical and computational simulation tools to show that transcriptional pausing at a site immediately downstream of a riboswitch requires a ligand-free pseudoknot in the nascent RNA, a precisely spaced consensus pause sequence, and electrostatic and steric interactions with the exit channel of bacterial RNA polymerase. We posit that many more examples of similarly intimate structural and kinetic coupling between RNA folding and gene expression remain to be discovered, leading to the exquisite regulatory control enabling all life processes. To reveal more such couplings, we will probe the dynamics of additional gene expression complexes using a tailored combination of single molecule fluorescence resonance energy transfer (smFRET) and Single Molecule Kinetic Analysis of RNA Transient Structure (SiM-KARTS). A major bottleneck in these pursuits so far has been the steep learning curve associated with our two home-built microscopes that keeps new group members from making significant contributions until they have completed 1- 2 years of training. We anticipate that addition of the ONI Nanoimager S to our microscopy arsenal will transform the speed of our progress by introducing an easy-to-use instrument that beginning postdocs, graduate and undergraduate students can quickly use independently until they ?graduate? to the home-built microscopes.

Public Health Relevance

Leveraging a portfolio of long-standing expertise at the interface of RNA biology and single molecule biophysics, the Walter group applies advanced mechanistic enzymology approaches to a broad set of RNAs involved in the regulation of transcription, translation and splicing, thus seizing the opportunities that continue to arise from discoveries of new functional RNAs. In addition, we will push the limits of our single molecule approaches to be able to probe increasingly complex biological contexts and mechanisms in which RNA structure governs the function of the cellular gene expression machinery. The acquisition of the proposed versatile, turnkey, easy-to- use ONI Nanoimager S fluorescence microscope will dramatically increase the throughput of our discovery pipeline as it will allow beginning postdocs, graduate students and undergraduate students alike to quickly climb the learning curve towards becoming productive group members.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
3R01GM062357-17S1
Application #
9894327
Study Section
Program Officer
Bender, Michael T
Project Start
2019-04-01
Project End
2020-12-31
Budget Start
2019-04-01
Budget End
2020-12-31
Support Year
17
Fiscal Year
2019
Total Cost
Indirect Cost

  Institution

Name
University of Michigan Ann Arbor
Department
Chemistry
Type
Schools of Arts and Sciences
DUNS #
073133571
City
Ann Arbor
State
MI
Country
United States
Zip Code
48109

  Publications

Johnson-Buck, Alexander; Li, Jieming; Tewari, Muneesh et al. (2018) A guide to nucleic acid detection by single-molecule kinetic fingerprinting. Methods :
Daher, May; Widom, Julia R; Tay, Wendy et al. (2018) Soft Interactions with Model Crowders and Non-canonical Interactions with Cellular Proteins Stabilize RNA Folding. J Mol Biol 430:509-523
Ray, Sujay; Widom, Julia R; Walter, Nils G (2018) Life under the Microscope: Single-Molecule Fluorescence Highlights the RNA World. Chem Rev 118:4120-4155
Daher, May; Mustoe, Anthony M; Morriss-Andrews, Alex et al. (2017) Tuning RNA folding and function through rational design of junction topology. Nucleic Acids Res 45:9706-9715
Michelini, Flavia; Pitchiaya, Sethuramasundaram; Vitelli, Valerio et al. (2017) Damage-induced lncRNAs control the DNA damage response through interaction with DDRNAs at individual double-strand breaks. Nat Cell Biol 19:1400-1411
Pitchiaya, Sethuramasundaram; Heinicke, Laurie A; Park, Jun I et al. (2017) Resolving Subcellular miRNA Trafficking and Turnover at Single-Molecule Resolution. Cell Rep 19:630-642
Suresh, Madathilparambil V; Thomas, Bivin; Machado-Aranda, David et al. (2016) Double-Stranded RNA Interacts With Toll-Like Receptor 3 in Driving the Acute Inflammatory Response Following Lung Contusion. Crit Care Med 44:e1054-e1066
Rinaldi, Arlie J; Lund, Paul E; Blanco, Mario R et al. (2016) The Shine-Dalgarno sequence of riboswitch-regulated single mRNAs shows ligand-dependent accessibility bursts. Nat Commun 7:8976
Bartke, Rebecca M; Cameron, Elizabeth L; Cristie-David, Ajitha S et al. (2015) Meeting report: SMART timing--principles of single molecule techniques course at the University of Michigan 2014. Biopolymers 103:296-302
Liberman, Joseph A; Suddala, Krishna C; Aytenfisu, Asaminew et al. (2015) Structural analysis of a class III preQ1 riboswitch reveals an aptamer distant from a ribosome-binding site regulated by fast dynamics. Proc Natl Acad Sci U S A 112:E3485-94

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