Abstract

To orchestrate neurotransmission, more than one thousand proteins are present at the presynaptic terminal and which either directly or indirectly interact with the synaptic vesicle. This high degree of convergence of presynaptic functions onto the synaptic vesicle has led to a ?vesicocentric? view of neurotransmission that focuses on the synaptic vesicle as the central organelle in synaptic function. As a result, much effort in molecular neurobiology in the past decades has been spent to identify the proteins present on synaptic vesicles and how they function to control neurotransmitter release. In addition, synaptic vesicles are also used as a model trafficking organelle to understand the mechanism utilized by the eukaryotic cell to carry out membrane fusion and trafficking. Because of these central roles synaptic vesicles play in neurotransmission as well as a model system for understanding membrane trafficking in general, it is critically important to develop a detailed and quantitative understanding of the organization of the synaptic vesicle. Synaptic vesicle is the smallest organelle present in the cell. From electron-microscopy (EM) measurements, synaptic vesicle has a diameter of ~40nm. In comparison, a ribosome observed under EM has a ?diameter? of 20-30nm depending on the contrast employed. In terms of size, therefore, synaptic vesicles are similar in many ways to a very large macromolecular complex, and as such, amenable to high- resolution single-molecule imaging and quantitative biophysical studies. Synaptic vesicle, however, is too large and disorganized to be studied with established structural methods, such as crystallography or cryoEM. The goal of the proposed project is to go beyond the compositional studies conducted in the past decade so as to unravel how proteins are spatially organized and interacting on the synaptic vesicle, and to construct a molecular/structural view of the synaptic vesicle. To achieve this, we have the following Aims:
Aim 1 : Single-Molecule Positional Mapping and Counting of Membrane Proteins on Synaptic Vesicles with Photoswitchable Pdots - this study will tell us which proteins are always located at the same positions on the vesicle, which proteins are adjacent to each other, and which are randomly distributed on the vesicle.
Aim 2 : Single-Molecule Orientation Mapping of Membrane Proteins on Synaptic Vesicles with Polarized Pdots - we know proteins are extremely crowded on the vesicle, but if proteins are interacting with each other or form a complex, then they are not only in close proximity but also would have the same rotational rate on the membrane or have very limited rotational freedom. This experiment will inform us which proteins are forming a complex and also whether they are in the same complex.
Aim 3 : Positional and Orientational Mapping of Membrane Proteins on Different Types of Synaptic Vesicle Enabled by a Nanoscale Sorter - different types of SVs might arrange the membrane proteins differently. We will use a nanoscale sorter to isolate and study different types of synaptic vesicles.

Public Health Relevance

Synaptic vesicle is the central organelle in neurotransmission. This project aims to develop a quantitative understanding of the organization of the synaptic vesicle, because unraveling how synaptic proteins are organized and constructing a molecularly precise picture of how the synaptic vesicle actually looks like will form the foundation from which to understand neurotransmission and synaptic function. A detailed molecular view of the synaptic vesicle will advance our understanding of the neural bases that underlies both normal physiology and pathophysiology that lead to mental illness.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Mental Health (NIMH)
Type
Research Project (R01)
Project #
5R01MH113333-04
Application #
9855075
Study Section
Special Emphasis Panel (ZRG1)
Program Officer
Driscoll, Jamie
Project Start
2017-03-01
Project End
2022-02-28
Budget Start
2020-03-01
Budget End
2021-02-28
Support Year
4
Fiscal Year
2020
Total Cost
Indirect Cost

  Institution

Name
University of Washington
Department
Chemistry
Type
Schools of Arts and Sciences
DUNS #
605799469
City
Seattle
State
WA
Country
United States
Zip Code
98195

  Publications

Jung, Seung-Ryoung; Han, Rui; Sun, Wei et al. (2018) Single-Molecule Flow Platform for the Quantification of Biomolecules Attached to Single Nanoparticles. Anal Chem 90:6089-6095
Jung, Seung-Ryoung; Fujimoto, Bryant S; Chiu, Daniel T (2017) Quantitative microscopy based on single-molecule fluorescence. Curr Opin Chem Biol 39:64-73
Wu, Li; Wu, I-Che; DuFort, Christopher C et al. (2017) Photostable Ratiometric Pdot Probe for in Vitro and in Vivo Imaging of Hypochlorous Acid. J Am Chem Soc 139:6911-6918
Kuo, Chun-Ting; Peng, Hong-Shang; Rong, Yu et al. (2017) Optically Encoded Semiconducting Polymer Dots with Single-Wavelength Excitation for Barcoding and Tracking of Single Cells. Anal Chem 89:6232-6238