The goal of this proposal is to develop a toolbox of genetically encoded indicators for biogenic amines, the most important family of neuromodulators. All nervous systems are subject to neuromodulation, which reconfigure the dynamics of neural circuitry by transforming the intrinsic firing properties of targeted neurons and regulating their synaptic plasticity. The altered dynamics of the neuromodulators have been implicated in a number of human neurological and psychiatric diseases, including Parkinson's, schizophrenia and addiction. Biogenic amines are a group of neuromodulators used by all animal brains to regulate the development, structure and function of neural circuits. Although the anatomical characterization and functional significance of biogenic amine projections are understood to a moderate degree, the precise mechanisms by which these molecules exert control over behavior are not fully understood. To decipher the mechanisms by which these molecules exert their influence on the brain and behavior, we must perform sensitive and specific measurements of neuromodulator transients, both broadly (volume modulation) and locally (targeted modulation), with the requisite spatial and temporal resolution, ideally in intac circuits. Existing methods, encompassing microdialysis and cyclic voltammetry, are useful, but not adequate for this task at hand. One potential solution would be to develop genetically encoded indicators based on fluorescent proteins combined with modern microscopy allowing direct and specific measurement of diverse types of neuromodulators with enhanced spatial and temporal resolutions. Recently we have successfully established technology platform for the development of genetically encoded indicators of neural activity, which have led to several high-quality optical probes for simultaneous imaging of large-scale neuronal populations in living animals. Building upon highly optimized platform for sensor sensors and extensive experience in sensor characterization and application in neuroscience, we propose to develop a high-quality toolkit of optical sensors for the biogenic amine neuromodulators, especially for dopamine, the most behavioral pervasive neuromodulator.
Our specific aims will start by designing and screening sensors for each of the biogenic amines using combined computational redesign and direct revolution. We will then develop synaptic targeting strategies to display the sensors in dendrites and axons to improve their utility for synaptic imaging. We will finally characterize the performance of these sensors in living neurons and in rat brain slices and demonstrate their capabilities of probing dynamics of dopamine transients in living animals. State-of-the-art sensors for these molecules will facilitate the non-invasive, precise, direct and continual measurement of released neuromodulators at both the synaptic and circuit levels in live model organisms. Such technology advance in optical recordings will facilitate neural circuitry mapping and paint a dynamic picture of neuromodulation systems in regulating neural circuitry and behavior. Given the clear relevance of the biogenic amines to the neurological diseases, these sensors are especially beneficial for long-term studies of human stem cell and animal disease models (specially the Parkinson's disease) and evaluating the effects of candidate therapeutics.

Public Health Relevance

The altered dynamics of the neuromodulators have been implicated in a number of human neurological and psychiatric diseases, including Parkinson's, schizophrenia and addiction. Our goal is to develop ultrasensitive genetically encoded sensors of the biogenic amines, the most powerful neuromodulators in the mammalian brain. Imaging the anatomical and functional organization of neuromodulation with these sensors in living model organisms will deepen our understanding of human neurological and psychiatric disorders and may bring us one step closer to finding improved treatment strategies.

Agency
National Institute of Health (NIH)
Institute
National Institute of Neurological Disorders and Stroke (NINDS)
Type
Research Project--Cooperative Agreements (U01)
Project #
3U01NS090604-02S1
Application #
9085037
Study Section
Special Emphasis Panel (ZNS1 (77))
Program Officer
Talley, Edmund M
Project Start
2014-09-30
Project End
2017-07-31
Budget Start
2015-08-01
Budget End
2016-07-31
Support Year
2
Fiscal Year
2015
Total Cost
$99,781
Indirect Cost
Name
University of California Davis
Department
Biochemistry
Type
Schools of Medicine
DUNS #
047120084
City
Davis
State
CA
Country
United States
Zip Code
95618
Broussard, Gerard Joey; Liang, Yajie; Fridman, Marina et al. (2018) In vivo measurement of afferent activity with axon-specific calcium imaging. Nat Neurosci 21:1272-1280
Patriarchi, Tommaso; Shen, Ao; He, Wei et al. (2018) Nanodelivery of a functional membrane receptor to manipulate cellular phenotype. Sci Rep 8:3556
Patriarchi, Tommaso; Cho, Jounhong Ryan; Merten, Katharina et al. (2018) Ultrafast neuronal imaging of dopamine dynamics with designed genetically encoded sensors. Science 360:
Corre, Julie; van Zessen, Ruud; Loureiro, Michaƫl et al. (2018) Dopamine neurons projecting to medial shell of the nucleus accumbens drive heroin reinforcement. Elife 7:
Mizuno, Grace O; Wang, Yinxue; Shi, Guilai et al. (2018) Aberrant Calcium Signaling in Astrocytes Inhibits Neuronal Excitability in a Human Down Syndrome Stem Cell Model. Cell Rep 24:355-365
Liang, Ruqiang; Broussard, Gerard Joseph; Tian, Lin (2015) Imaging chemical neurotransmission with genetically encoded fluorescent sensors. ACS Chem Neurosci 6:84-93
Broussard, Gerard J; Liang, Ruqiang; Tian, Lin (2014) Monitoring activity in neural circuits with genetically encoded indicators. Front Mol Neurosci 7:97