Abstract

A critical gap remains in our understanding of oxygen metabolism, delivery, and reserve, both at rest and during metabolic activation states in healthy and diseased brain. Available imaging techniques lack spatial and temporal resolution to assess distribution of cerebral tissue oxygenation (PO2) and O2 consumption (CMRO2) with adequate level of detail, and to unravel their dynamic changes within microvascular domains. We propose to develop and validate a new microscopic imaging method of resting state CMRO2 in small animal models, and advance it to enable rapid high spatial resolution imaging of CMRO2 and PO2. The new technology will enable regional estimation of CMRO2 at a rate of ~1 Hz together with acquisition of detailed tissue PO2 maps, which is essential for advancing our understanding of O2 delivery and consumption in the brain.
In Aim1 we will develop and validate high-resolution resting state CMRO2 imaging method in small rodents based on two- photon PO2 microscopy. This new method will measure resting state regional CMRO2 based on tissue PO2 profiles around cortical penetrating arterioles.
In Aim 2 we will advance new CMRO2 imaging method by improving a multifocal, frequency modulated, two-photon phosphorescence lifetime imaging to allow practical rapid PO2 imaging in optically scattering brain tissue, and to improve the speed of CMRO2 measurements up to 100-fold (approaching 1 Hz).
In Aim 3 we will quantify regional CMRO2 during physiological and pathological perturbations. We will test the hypothesis that transient physiological or pathological neuronal activation in a brain affected by ischemia leads to a mismatch between O2 metabolism and supply and hypoxia within microvascular domains - a mechanism that may underlie lesion growth in stroke and other brain injury states as well as progressive neurodegeneration observed in microvasculopathies. This technology will have broad utility in quantifying metabolism and oxygenation in cerebral microvascular domains in animal models of brain disorders that will dramatically advance our understanding of pathophysiology and lead to novel treatment strategies in important clinical problems such as chronic cerebral hypoperfusion, stroke, small vessel disease, and AD dementia.

Public Health Relevance

High spatiotemporal resolution microscopy imaging of cerebral oxygen metabolism and tissue oxygenation will enable quantitative characterization of the influences of oxygen supply and consumption on availability of oxygen in microvascular domains. This will be an imaging approach that will have broad utility in quantifying the metabolism and oxygenation in cerebral micro domains in animal models of brain disorders that will dramatically advance our understanding of pathophysiology and lead to novel treatment strategies in important clinical problems such as stroke, chronic cerebral hypoperfusion, small vessel disease, and AD dementia. The utility will be applied to test the hypothesis that transient physiological or pathological neuronal activation in ischemic brain leads to a mismatch between oxygen supply and consumption and hypoxia within microvascular domains.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Neurological Disorders and Stroke (NINDS)
Type
Research Project (R01)
Project #
1R01NS091230-01A1
Application #
8985334
Study Section
Neuroscience and Ophthalmic Imaging Technologies Study Section (NOIT)
Program Officer
Babcock, Debra J
Project Start
2015-07-15
Project End
2020-05-31
Budget Start
2015-07-15
Budget End
2016-05-31
Support Year
1
Fiscal Year
2015
Total Cost
Indirect Cost

  Institution

Name
Massachusetts General Hospital
Department
Type
DUNS #
073130411
City
Boston
State
MA
Country
United States
Zip Code

  Publications

Kura, Sreekanth; Xie, Hongyu; Fu, Buyin et al. (2018) Intrinsic optical signal imaging of the blood volume changes is sufficient for mapping the resting state functional connectivity in the rodent cortex. J Neural Eng 15:035003
Chung, David Y; Sadeghian, Homa; Qin, Tao et al. (2018) Determinants of Optogenetic Cortical Spreading Depolarizations. Cereb Cortex :
Tang, Jianbo; Erdener, Sefik Evren; Li, Baoqiang et al. (2018) Shear-induced diffusion of red blood cells measured with dynamic light scattering-optical coherence tomography. J Biophotonics 11:
Chung, David Y; Sugimoto, Kazutaka; Fischer, Paul et al. (2018) Real-time non-invasive in vivo visible light detection of cortical spreading depolarizations in mice. J Neurosci Methods 309:143-146
Gómez, Carlos A; Sutin, Jason; Wu, Weicheng et al. (2018) Phasor analysis of NADH FLIM identifies pharmacological disruptions to mitochondrial metabolic processes in the rodent cerebral cortex. PLoS One 13:e0194578
Pouliot, Philippe; Gagnon, Louis; Lam, Tina et al. (2017) Magnetic resonance fingerprinting based on realistic vasculature in mice. Neuroimage 149:436-445
Rasmussen, Peter M; Smith, Amy F; Sakadži?, Sava et al. (2017) Model-based inference from microvascular measurements: Combining experimental measurements and model predictions using a Bayesian probabilistic approach. Microcirculation 24:
Yaseen, Mohammad A; Sutin, Jason; Wu, Weicheng et al. (2017) Fluorescence lifetime microscopy of NADH distinguishes alterations in cerebral metabolism in vivo. Biomed Opt Express 8:2368-2385
Kisler, Kassandra; Nelson, Amy R; Rege, Sanket V et al. (2017) Pericyte degeneration leads to neurovascular uncoupling and limits oxygen supply to brain. Nat Neurosci 20:406-416
Li, Baoqiang; Wang, Hui; Fu, Buyin et al. (2017) Impact of temporal resolution on estimating capillary RBC-flux with optical coherence tomography. J Biomed Opt 22:16014

Showing the most recent 10 out of 25 publications