Abstract

Ca2+ ions serve as a signaling mechanism in almost all cell types to regulate numerous diverse functions. Ca2+ signals are ordered in a hierarchy, from openings of single Ca2+ channels ('fundamental' events), through the concerted openings of clustered channels ('elementary' events, such as Ca2+ puffs) to propagating Ca2+ waves, coordinated through Ca2+ diffusion and Ca2+-induced Ca2+ release. Fundamental and elementary events thus form the triggers and building blocks underlying the complex spatiotemporal Ca2+ signals that permit graded and selective regulation of cell functions. Our overall goals are to elucidate how the functional properties, spatial organization and interactions between Ca2-t- channels pattern spatiotemporal cellular signals. We focus on Ca2+ events underlying the inositol trisphosphate (IP3) signaling pathway, and Ca2+ flux through amyloid oligomer pores implicated in the pathophysiology of Alzheimer's disease. Capitalizing on recent advances in biophotonic technology, including total intemal reflection fluorescence and superresolution microscopy, we can now study these topics at the truly single- molecule level in intact cells.
Our aims are to: (i) Further develop techniques for fast, 3-dimensional imaging Ca2+ flux through individual IPS receptor/channels (IP3Rs) in intact cells; for monitoring ER [Ca2+]; and for single-molecule localization of subtypes of native IP3Rs in transgenic mouse models, (ii) Elucidate the functional properties of IP3Rs in the intact cell, how the activity of channels is orchestrated to generate and temiinate elementary Ca2+ puffs, and to generate global Ca2+ waves, (iii) Resolve IP3R molecules with sub-micron precision to address hypotheses concerning the clustered organization and anchoring of these channels; their interactions via Ca2+ diffusion and allosteric mechanisms; and the putative function of 'silenf IP3Rs between puff sites, (iv) Investigate the molecular mechanisms by which amyloid oligomers form Ca2+- permeable pores by combining single-channel Ca2+ imaging with single-molecule photobleaching of fluorescent monomers to detennine pore stoichiometry; and elucidate the mechanisms by which intracellular oligomers induce Ca2+ liberation through IP3Rs.

Public Health Relevance

Calcium sen/es a 'life or death' function in virtually all cells ofthe body, regulating processes as diverse as the heartbeat and synaptic transmission between brain cells, and is implicated in Alzheimer's and other diseases. Our goal is to elucidate the hierarchical mechanisms by which calcium signals are generated at the single-molecule level, with the dual aims of better understanding their normal functioning and how disruntions in r-alrJum signaling mav lead to disease.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Method to Extend Research in Time (MERIT) Award (R37)
Project #
4R37GM048071-25
Application #
9036691
Study Section
Special Emphasis Panel (NSS)
Program Officer
Nie, Zhongzhen
Project Start
1992-08-01
Project End
2021-08-31
Budget Start
2016-09-01
Budget End
2017-08-31
Support Year
25
Fiscal Year
2016
Total Cost
Indirect Cost

  Institution

Name
University of California Irvine
Department
Type
DUNS #
046705849
City
Irvine
State
CA
Country
United States
Zip Code
92617

  Publications

Ma, Zhongming; Taruno, Akiyuki; Ohmoto, Makoto et al. (2018) CALHM3 Is Essential for Rapid Ion Channel-Mediated Purinergic Neurotransmission of GPCR-Mediated Tastes. Neuron 98:547-561.e10
Ellefsen, Kyle L; Parker, Ian (2018) Dynamic Ca2+ imaging with a simplified lattice light-sheet microscope: A sideways view of subcellular Ca2+ puffs. Cell Calcium 71:34-44
Lock, Jeffrey T; Alzayady, Kamil J; Yule, David I et al. (2018) All three IP3 receptor isoforms generate Ca2+ puffs that display similar characteristics. Sci Signal 11:
Shah, Syed Islamuddin; Demuro, Angelo; Mak, Don-On Daniel et al. (2018) TraceSpecks: A Software for Automated Idealization of Noisy Patch-Clamp and Imaging Data. Biophys J 115:9-21
Ellefsen, Kyle L; Lock, Jeffrey T; Settle, Brett et al. (2018) Applications of FLIKA, a Python-based image processing and analysis platform, for studying local events of cellular calcium signaling. Biochim Biophys Acta Mol Cell Res :
Dong, Tobias X; Othy, Shivashankar; Jairaman, Amit et al. (2017) T-cell calcium dynamics visualized in a ratiometric tdTomato-GCaMP6f transgenic reporter mouse. Elife 6:
Parker, Ian; Evans, Katrina T; Ellefsen, Kyle et al. (2017) Lattice light sheet imaging of membrane nanotubes between human breast cancer cells in culture and in brain metastases. Sci Rep 7:11029
Dong, Tobias X; Othy, Shivashankar; Greenberg, Milton L et al. (2017) Intermittent Ca2+ signals mediated by Orai1 regulate basal T cell motility. Elife 6:
Lock, Jeffrey T; Smith, Ian F; Parker, Ian (2017) Comparison of Ca2+puffs evoked by extracellular agonists and photoreleased IP3. Cell Calcium 63:43-47
Dickinson, George D; Ellefsen, Kyle L; Dawson, Silvina Ponce et al. (2016) Hindered cytoplasmic diffusion of inositol trisphosphate restricts its cellular range of action. Sci Signal 9:ra108

Showing the most recent 10 out of 51 publications