Literature DB >> 28663879

Fluorescence lifetime microscopy of NADH distinguishes alterations in cerebral metabolism in vivo.

Mohammad A Yaseen1, Jason Sutin1, Weicheng Wu1, Buyin Fu1, Hana Uhlirova2,3, Anna Devor1,2, David A Boas1, Sava Sakadžić1.   

Abstract

Evaluating cerebral energy metabolism at microscopic resolution is important for comprehensively understanding healthy brain function and its pathological alterations. Here, we resolve specific alterations in cerebral metabolism in vivo in Sprague Dawley rats utilizing minimally-invasive 2-photon fluorescence lifetime imaging (2P-FLIM) measurements of reduced nicotinamide adenine dinucleotide (NADH) fluorescence. Time-resolved fluorescence lifetime measurements enable distinction of different components contributing to NADH autofluorescence. Ostensibly, these components indicate different enzyme-bound formulations of NADH. We observed distinct variations in the relative proportions of these components before and after pharmacological-induced impairments to several reactions involved in glycolytic and oxidative metabolism. Classification models were developed with the experimental data and used to predict the metabolic impairments induced during separate experiments involving bicuculline-induced seizures. The models consistently predicted that prolonged focal seizure activity results in impaired activity in the electron transport chain, likely the consequence of inadequate oxygen supply. 2P-FLIM observations of cerebral NADH will help advance our understanding of cerebral energetics at a microscopic scale. Such knowledge will aid in our evaluation of healthy and diseased cerebral physiology and guide diagnostic and therapeutic strategies that target cerebral energetics.

Entities:  

Keywords:  (170.0170) Medical optics and biotechnology; (170.3650) Lifetime-based sensing; (180.4315) Nonlinear microscopy

Year:  2017        PMID: 28663879      PMCID: PMC5480486          DOI: 10.1364/BOE.8.002368

Source DB:  PubMed          Journal:  Biomed Opt Express        ISSN: 2156-7085            Impact factor:   3.732


  67 in total

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Journal:  Opt Express       Date:  2008-03-17       Impact factor: 3.894

4.  Nicotinamide adenine dinucleotides in the developing rat brain.

Authors:  R Guarneri; V Bonavita
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5.  Preictal and ictal neurovascular and metabolic coupling surrounding a seizure focus.

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6.  In vivo optical mapping of epileptic foci and surround inhibition in ferret cerebral cortex.

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7.  Glycolysis and epilepsy-induced changes in cerebrocortical NAD/NADH redox state.

Authors:  E Dóra
Journal:  J Neurochem       Date:  1983-12       Impact factor: 5.372

8.  Time-resolved spectroscopic imaging reveals the fundamentals of cellular NADH fluorescence.

Authors:  Dong Li; Wei Zheng; Jianan Y Qu
Journal:  Opt Lett       Date:  2008-10-15       Impact factor: 3.776

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10.  Initiation of spontaneous epileptiform events in the rat neocortex in vivo.

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  25 in total

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Review 2.  Evaluating Cell Metabolism Through Autofluorescence Imaging of NAD(P)H and FAD.

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Journal:  Antioxid Redox Signal       Date:  2018-01-30       Impact factor: 8.401

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4.  In vivo imaging and analysis of cerebrovascular hemodynamic responses and tissue oxygenation in the mouse brain.

Authors:  Kassandra Kisler; Divna Lazic; Melanie D Sweeney; Shane Plunkett; Mirna El Khatib; Sergei A Vinogradov; David A Boas; Sava Sakadži; Berislav V Zlokovic
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6.  In vivo fluorescence lifetime imaging of macrophage intracellular metabolism during wound responses in zebrafish.

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7.  NAD(P)H autofluorescence lifetime imaging enables single cell analyses of cellular metabolism of osteoblasts in vitro and in vivo via two-photon microscopy.

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8.  Drosophila TRIM32 cooperates with glycolytic enzymes to promote cell growth.

Authors:  Simranjot Bawa; David S Brooks; Kathryn E Neville; Marla Tipping; Md Abdul Sagar; Joseph A Kollhoff; Geetanjali Chawla; Brian V Geisbrecht; Jason M Tennessen; Kevin W Eliceiri; Erika R Geisbrecht
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9.  Autofluorescence lifetime imaging of cellular metabolism: Sensitivity toward cell density, pH, intracellular, and intercellular heterogeneity.

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10.  Label-free fluorescence lifetime spectroscopy detects radiation-induced necrotic changes in live brain in real-time.

Authors:  Brad A Hartl; Htet S W Ma; Shamira Sridharan; Katherine S Hansen; Michael S Kent; Fredric Gorin; Ruben C Fragoso; Laura Marcu
Journal:  Biomed Opt Express       Date:  2018-07-05       Impact factor: 3.732

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