Abstract

Presynaptic terminals are fundamental computational units in the brain, and their dysfunction is associated with several neurological diseases. They mediate the transduction of incoming electrical signals (action potentials) into chemical signals (neurotransmitter release), and the efficiency of conversion determines the strength of circuits underlying memory and behavior. The ultimate goal of this proposal is to understand the mechanisms by which presynaptic cellular machineries modulate the electro-chemical transduction of action potentials. It is known that presynaptic terminals are highly adaptive structures capable of maintaining transmission across vastly different input rates, metabolic states, and vesicle fusion probabilities. Our recent work in combination with others has exposed the fact that action potentials are not invariant signals. One critical level of regulation exists within the axonal arborization, which actively regulates the propagation and shape of electrical signals arriving at each of its presynaptic terminals. We hypothesize that a second complementary, but currently uncharacterized, set of mechanisms exist at presynaptic terminals that rapidly sense the cellular state and alter the chemical transduction of electrical signal inputs. As a result, the individual presynaptic terminals instantaneously adjust the electrogenic properties of their membranes through local ion channel activation pathways which dynamically regulate the chemical response to a given action potential as it arrives. We propose to identify the molecular basis of this ?on the fly? control system of transduction in the following aims:
Aim 1. We will determine how the cellular metabolic energy state of the synapse (ATP:ADP ratio) influences action potential transduction via ATP-sensitive potassium channels.
Aim 2. We will determine how stimulation frequency alters the activation of presynaptic voltage- and calciumsensitive potassium channels to influence action potential transduction in excitatory and inhibitory terminals.
Aim 3. We will determine how coupling calcium channels to vesicle fusion release machinery controls potassium channel activation. Results from these aims will present new data on electrogenic mechanisms influencing complex computations of presynaptic terminals, leading to a more complete understanding of synaptic plasticity and neuronal processing.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Exploratory Grants (P20)
Project #
5P20GM113132-05
Application #
10215732
Study Section
Special Emphasis Panel (ZGM1)
Program Officer
Davani, Behrous
Project Start
2018-03-01
Project End
2021-02-28
Budget Start
2020-03-01
Budget End
2021-02-28
Support Year
5
Fiscal Year
2020
Total Cost
Indirect Cost

  Institution

Name
Dartmouth College
Department
Type
DUNS #
041027822
City
Hanover
State
NH
Country
United States
Zip Code
03755

  Publications

Cabrera, Jorge Ruben; Charron, Audra J; Leib, David A (2018) Neuronal subtype determines HSV-1 Latency-Associated-Transcript (LAT) promoter activity during latency. J Virol :
Olmedillas, Eduardo; Cano, Olga; Martínez, Isidoro et al. (2018) Chimeric Pneumoviridae fusion proteins as immunogens to induce cross-neutralizing antibody responses. EMBO Mol Med 10:175-187
Hvorecny, Kelli L; Dolben, Emily; Moreau-Marquis, Sophie et al. (2018) An epoxide hydrolase secreted by Pseudomonas aeruginosa decreases mucociliary transport and hinders bacterial clearance from the lung. Am J Physiol Lung Cell Mol Physiol 314:L150-L156
Holland, Jack; Pan, Qinxin; Grigoryan, Gevorg (2018) Contact prediction is hardest for the most informative contacts, but improves with the incorporation of contact potentials. PLoS One 13:e0199585
Young, Lorna E; Higgs, Henry N (2018) Focal Adhesions Undergo Longitudinal Splitting into Fixed-Width Units. Curr Biol 28:2033-2045.e5
Kettenbach, Arminja N; Schlosser, Kate A; Lyons, Scott P et al. (2018) Global assessment of its network dynamics reveals that the kinase Plk1 inhibits the phosphatase PP6 to promote Aurora A activity. Sci Signal 11:
Lyons, Scott P; Jenkins, Nicole P; Nasa, Isha et al. (2018) A Quantitative Chemical Proteomic Strategy for Profiling Phosphoprotein Phosphatases from Yeast to Humans. Mol Cell Proteomics 17:2447-2461
Bricio-Moreno, Laura; Sheridan, Victoria H; Goodhead, Ian et al. (2018) Evolutionary trade-offs associated with loss of PmrB function in host-adapted Pseudomonas aeruginosa. Nat Commun 9:2635
Kumar, Ganesan Senthil; Choy, Meng S; Koveal, Dorothy M et al. (2018) Identification of the substrate recruitment mechanism of the muscle glycogen protein phosphatase 1 holoenzyme. Sci Adv 4:eaau6044
Xia, Xue; Katzenell, Sarah; Reinhart, Erin F et al. (2018) A pseudo-receiver domain in Atg32 is required for mitophagy. Autophagy 14:1620-1628

Showing the most recent 10 out of 56 publications