Literature DB >> 22029350

Two-photon microscopy of cortical NADH fluorescence intensity changes: correcting contamination from the hemodynamic response.

Edward Baraghis1, Anna Devor, Qianqian Fang, Vivek J Srinivasan, Weicheng Wu, Frédéric Lesage, Cenk Ayata, Karl A Kasischke, David A Boas, Sava Sakadzić.   

Abstract

Quantification of nicotinamide adenine dinucleotide (NADH) changes during functional brain activation and pathological conditions provides critical insight into brain metabolism. Of the different imaging modalities, two-photon laser scanning microscopy (TPLSM) is becoming an important tool for cellular-resolution measurements of NADH changes associated with cellular metabolic changes. However, NADH fluorescence emission is strongly absorbed by hemoglobin. As a result, in vivo measurements are significantly affected by the hemodynamics associated with physiological and pathophysiological manipulations. We model NADH fluorescence excitation and emission in TPLSM imaging based on precise maps of cerebral microvasculature. The effects of hemoglobin optical absorption and optical scattering from red blood cells, changes in blood volume and hemoglobin oxygen saturation, vessel size, and location with respect to imaging location are explored. A simple technique for correcting the measured NADH fluorescence intensity changes is provided, with the utilization of a parallel measurement of a physiologically inert fluorophore. The model is applied to TPLSM measurements of NADH fluorescence intensity changes in rat somatosensory cortex during mild hypoxia and hyperoxia. The general approach of the correction algorithm can be extended to other TPLSM measurements, where changes in the optical properties of the tissue confound physiological measurements, such as the detection of calcium dynamics.

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Year:  2011        PMID: 22029350      PMCID: PMC3206923          DOI: 10.1117/1.3633339

Source DB:  PubMed          Journal:  J Biomed Opt        ISSN: 1083-3668            Impact factor:   3.170


  45 in total

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Review 2.  Microvascular rheology and hemodynamics.

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Journal:  Microcirculation       Date:  2005 Jan-Feb       Impact factor: 2.628

3.  Influence of optical properties on two-photon fluorescence imaging in turbid samples.

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Journal:  Appl Opt       Date:  2000-03-01       Impact factor: 1.980

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5.  Intracellular redox changes in functioning cerebral cortex. I. Metabolic effects of epileptiform activity.

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6.  Oxidation of NADH during contractions of circulated mammalian skeletal muscle.

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Journal:  Respir Physiol       Date:  1968-05

7.  Sulforhodamine 101 as a specific marker of astroglia in the neocortex in vivo.

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8.  Two-photon autofluorescence dynamics imaging reveals sensitivity of intracellular NADH concentration and conformation to cell physiology at the single-cell level.

Authors:  Qianru Yu; Ahmed A Heikal
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9.  Cortical spreading depression causes and coincides with tissue hypoxia.

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10.  Two-photon NADH imaging exposes boundaries of oxygen diffusion in cortical vascular supply regions.

Authors:  Karl A Kasischke; Elton M Lambert; Ben Panepento; Anita Sun; Harris A Gelbard; Robert W Burgess; Thomas H Foster; Maiken Nedergaard
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  12 in total

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3.  Physiology-based kinetic modeling of neuronal energy metabolism unravels the molecular basis of NAD(P)H fluorescence transients.

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

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Journal:  Nat Protoc       Date:  2018-05-24       Impact factor: 13.491

Review 5.  High-resolution in vivo optical imaging of stroke injury and repair.

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6.  Brain Tissue PO2 Measurement During Normoxia and Hypoxia Using Two-Photon Phosphorescence Lifetime Microscopy.

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7.  In vivo imaging of cerebral energy metabolism with two-photon fluorescence lifetime microscopy of NADH.

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8.  Pericyte degeneration leads to neurovascular uncoupling and limits oxygen supply to brain.

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Journal:  Nat Neurosci       Date:  2017-01-30       Impact factor: 24.884

9.  Intravital imaging in spontaneously hypertensive stroke-prone rats-a pilot study.

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Review 10.  Contributions and complexities from the use of in vivo animal models to improve understanding of human neuroimaging signals.

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