Abstract

Since the genetic code was elucidated in the early 1960's, it has been assumed that mRNAs are always decoded in three base codons, that any deviation from this fundamental rule must be erroneous and thus, deleterious. However, over the past decade, we have shown that a significant fraction of cellular mRNAs harbor cis-acting sequence elements that direct elongating ribosomes to shift reading frame by one base in the 5' (-1) direction. In cellular mRNAs, such Programmed -1 Ribosomal Frameshift (-1 PRF) signals direct ribosomes to premature termination codons where they become substrates for rapid degradation through the Nonsense-Mediated mRNA Decay (NMD) pathway, resulting in decreased expression of the proteins encoded by these mRNAs. Importantly, rates of mRNA degradation are proportional to rates of -1 PRF, a relationship that is conserved in eukaryotes from yeast to humans. Observations from yeast to humans that global changes in -1 PRF rates are deleterious to cellular function suggested that regulation of -1 PRF must be sequence- specific. Recently, we discovered that this is achieved through the interactions between -1 PRF signals and miRNAs. These findings have initiated a completely new avenue of research by establishing -1 PRF on cellular mRNAs, and its regulation by miRNAs as a new, fundamental paradigm in gene expression. This proposal seeks to deepen our understanding of the molecular mechanisms underlying regulation of -1 PRF in human cells. The well-defined Jurkat human T-cell line and a focus on -1 PRF signals embedded in mRNAs encoding cytokine receptors and a critical cytokine-responsive tyrosine kinase provides a model system to address a series of questions ranging from basic molecular and structural biology to regulation and control of the acquired immune response.
Aim 1 of this proposal seeks to confirm -1 PRF promoted by sequences identified in the mRNAs encoding IL2R?, IL7R?, and JAK2, characterize the effects of SNPs on -1 PRF, and develop the next generation PRF technology.
Aim 2 will identify and validate miRNAs that naturally interact with these -1 PRF signals, and will test an autoregulatory feedback loop model of -1 PRF.
Aim 3 is oriented towards characterizing the effects of miRNAs on gene expression and RNA structure. By the end of the proposed studies, we will have 1) deepened our understanding of this new paradigm gene expression control, 2) identified specific miRNAs that are used by T-cells to control their responses to important cytokines, and 3) established new rules describing mRNA/miRNA atomic scale structural interactions. These studies will immediately impact many fields including basic molecular and cell biology, and more applied fields including immunology and HIV/AIDS, and will lay the foundation for the design and discovery of small molecule therapeutics targeted to specific -1 PRF signals.

Public Health Relevance

Programmed -1 ribosomal frameshifting (-1 PRF) is a fundamental molecular mechanism that is used to control gene expression from yeast to humans by destabilizing messenger RNAs. Building on our recent demonstration of sequence-specific regulation of -1 PRF by micro-RNAs (miRNAs), we will identify the miRNAs that are naturally used by cells to regulate -1 PRF in a subset of mRNAs involved in cytokine responses of human T-cells, and will characterize the relationship between mRNA/miRNA structures on -1 PRF and gene expression. The studies proposed in this application will expand our understanding of RNA structure/function relationships and lay the foundation for the design of small molecule therapeutics targeted to specific -1 PRF signals.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM117177-03
Application #
9278237
Study Section
Molecular Genetics B Study Section (MGB)
Program Officer
Sledjeski, Darren D
Project Start
2015-09-25
Project End
2019-05-31
Budget Start
2017-06-01
Budget End
2018-05-31
Support Year
3
Fiscal Year
2017
Total Cost
Indirect Cost

  Institution

Name
University of Maryland College Park
Department
Anatomy/Cell Biology
Type
Earth Sciences/Resources
DUNS #
790934285
City
College Park
State
MD
Country
United States
Zip Code
20742

  Publications

Kendra, Joseph A; Advani, Vivek M; Chen, Bin et al. (2018) Functional and structural characterization of the chikungunya virus translational recoding signals. J Biol Chem 293:17536-17545
Dever, Thomas E; Dinman, Jonathan D; Green, Rachel (2018) Translation Elongation and Recoding in Eukaryotes. Cold Spring Harb Perspect Biol 10:
Chen, Bin; Longhini, Andrew P; Nußbaumer, Felix et al. (2018) CCR5 RNA Pseudoknots: Residue and Site-Specific Labeling correlate Internal Motions with microRNA Binding. Chemistry 24:5462-5468
Girardi, T; Vereecke, S; Sulima, S O et al. (2018) The T-cell leukemia-associated ribosomal RPL10 R98S mutation enhances JAK-STAT signaling. Leukemia 32:809-819
Briggs, Joseph W; Dinman, Jonathan D (2017) Subtractional Heterogeneity: A Crucial Step toward Defining Specialized Ribosomes. Mol Cell 67:3-4
Sulima, Sergey O; Hofman, Isabel J F; De Keersmaecker, Kim et al. (2017) How Ribosomes Translate Cancer. Cancer Discov 7:1069-1087
Gulay, Suna P; Bista, Sujal; Varshney, Amitabh et al. (2017) Tracking fluctuation hotspots on the yeast ribosome through the elongation cycle. Nucleic Acids Res 45:4958-4971
Meydan, Sezen; Klepacki, Dorota; Karthikeyan, Subbulakshmi et al. (2017) Programmed Ribosomal Frameshifting Generates a Copper Transporter and a Copper Chaperone from the Same Gene. Mol Cell 65:207-219
Briggs, Joseph W; Ren, Ling; Chakrabarti, Kristi R et al. (2017) Activation of the unfolded protein response in sarcoma cells treated with rapamycin or temsirolimus. PLoS One 12:e0185089
Paolini, Nahuel A; Attwood, Martin; Sondalle, Samuel B et al. (2017) A Ribosomopathy Reveals Decoding Defective Ribosomes Driving Human Dysmorphism. Am J Hum Genet 100:506-522

Showing the most recent 10 out of 17 publications