The physiological effects of cocaine are mediated by inhibition of dopamine reuptake, and subsequent enhancement of dopaminergic neurotransmission. We recently made a surprising and unexpected finding that physiological effects of cocaine in animals requires methylation of adenosine residues in mRNA. Adenosine methylation constitutes the first, and potentially only, reversible mRNA modification. Last year, our group showed that methylation of adenosine residues in mRNA to form N6-methyladenosine (m6A) is highly prevalent and affects over 8,000 transcripts in the brain. Furthermore, adenosine methylation and demethylation is regulated by signaling pathways, suggesting that adenosine methylation, like protein phosphorylation, may be a fundamental mechanism mediating effects of signaling pathways in cells. The goal of this application is to substantially advance our understanding of this newly discovered and largely mysterious mRNA modification that appears to have a central role in synaptic transmission and neuronal function. As part of our overall goal to understand the cellular functions of m6A and to determine how it regulates dopaminergic neurotransmission, the specific aims of this proposal are: (1) To map m6A sites in the midbrain transcriptome at single-nucleotide resolution. We will develop a next-generation sequencing approach that uses a novel to detect m6A in living cells. These experiments will provide new insights into the potential biological functions of m6A and will result in the identification of m6A sites in the midbrain transcriptome for analysis and mutagenesis in Aims 2; (2) To determine how m6A regulates protein translation in neurons. We will explore the relationship between m6A and protein translation and determine the structural and sequence contexts that enable m6A to influence mRNA translation in vitro and in neurons. We will also determine the specific m6A-binding proteins that mediate the effects of m6A on mRNA translation; (3) We will determine how FTO controls translation via its ability to demethylate m6A. We find that FTO selectively demethylates m6A residues in vivo. We will test the hypothesis that FTO reprograms protein translation pathways in neurons by influencing the translation of specific transcripts relevant to dopaminergic neurotransmission. The experiments proposed here will provide fundamentally novel insights into how neuronal protein translation is regulated. The pathways described here are likely to influence diverse aspects of neuronal function. These experiments will begin to decipher the role of a novel, highly prevalent, and brain-enriched mRNA modification that is poised to have important roles in dopamine neurotransmission as well as other signaling pathways in neurons and other tissues.

Public Health Relevance

We recently found that animals that are deficient in the FTO gene, which demethylates adenosine residues in specific mRNAs, are nearly resistant to the motor and synaptic signaling effects of cocaine and have other synaptic signaling defects in dopaminergic neurons. In this application, we propose experiments to uncover how adenosine methylation and FTO control neuron function by: (1) developing novel techniques for precisely localizing the residues that are methylated at a transcriptome-wide level; (2) by determining how methylated adenosine affects mRNA translation; and (3) by identifying how FTO controls patterns of translation in dopaminergic neurons. These experiments seek to provide an explanation for the function of FTO and adenosine methylation in neurons, and thereby provide a basis for beginning to understand how this pathway can influence dopaminergic signaling and the responses of animals to cocaine.

Agency
National Institute of Health (NIH)
Institute
National Institute on Drug Abuse (NIDA)
Type
Research Project (R01)
Project #
5R01DA037755-05
Application #
9493455
Study Section
Special Emphasis Panel (ZRG1)
Program Officer
Satterlee, John S
Project Start
2014-06-01
Project End
2019-05-31
Budget Start
2018-06-01
Budget End
2019-05-31
Support Year
5
Fiscal Year
2018
Total Cost
Indirect Cost
Name
Weill Medical College of Cornell University
Department
Pharmacology
Type
Schools of Medicine
DUNS #
060217502
City
New York
State
NY
Country
United States
Zip Code
10065
Patil, Deepak P; Pickering, Brian F; Jaffrey, Samie R (2018) Reading m6A in the Transcriptome: m6A-Binding Proteins. Trends Cell Biol 28:113-127
Grozhik, Anya V; Linder, Bastian; Olarerin-George, Anthony O et al. (2017) Mapping m6A at Individual-Nucleotide Resolution Using Crosslinking and Immunoprecipitation (miCLIP). Methods Mol Biol 1562:55-78
Meyer, Kate D; Jaffrey, Samie R (2017) Rethinking m6A Readers, Writers, and Erasers. Annu Rev Cell Dev Biol 33:319-342
Mauer, Jan; Luo, Xiaobing; Blanjoie, Alexandre et al. (2017) Reversible methylation of m6Am in the 5' cap controls mRNA stability. Nature 541:371-375
Meyer, Kate D; Patil, Deepak P; Zhou, Jun et al. (2015) 5' UTR m(6)A Promotes Cap-Independent Translation. Cell 163:999-1010
Meyer, Kate D; Jaffrey, Samie R (2014) The dynamic epitranscriptome: N6-methyladenosine and gene expression control. Nat Rev Mol Cell Biol 15:313-26
Jaffrey, Samie R (2014) An expanding universe of mRNA modifications. Nat Struct Mol Biol 21:945-6